An object of the present invention is to provide a separation agent for separating a human serum-derived IgG polyclonal antibody. This object is achieved by a separation agent for separating a human serum-derived IgG polyclonal antibody, the separation agent including: a carrier; and a single-chain antibody which has a dissociation constant for a human serum-derived IgG polyclonal antibody of not more than 3.0×10−8 M and which binds to the surface of the carrier via a chemical bond.
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1. A separation agent for separating a human serum-derived IgG polyclonal antibody, the separation agent comprising: a carrier; and a single-chain antibody which has a dissociation constant for a human serum-derived IgG polyclonal antibody of not more than 3.0×10−8 M and which binds to the surface of the carrier via a chemical bond,
wherein the single-chain antibody is selected from the following single-chain antibodies (a) to (e):
(a) the single-chain antibody having
the amino acid sequence of the heavy-chain CDR3: ATRYDSYGYAYNYWFGTLW (SEQ ID NO: 148);
wherein the single-chain antibody (a) further comprises the following amino acid sequence (a-1) or (a-2):
(a-1) the amino acid sequence of the heavy-chain CDR1: SGIDLSSNA (SEQ ID NO: 153),
the amino acid sequence of the heavy-chain CDR2: ISTVGKT (SEQ ID NO: 154),
the amino acid sequence of the light-chain CDR1: ENINSE (SEQ ID NO: 155),
the amino acid sequence of the light-chain CDR2: DAS, and
the amino acid sequence of the light-chain CDR3: QSTYYDGNYVYA (SEQ ID NO: 156); and
(a-2) the amino acid sequence of the heavy-chain CDR1: SGIDLSSNA (SEQ ID NO: 153),
the amino acid sequence of the heavy-chain CDR2: ISTGGST (SEQ ID NO: 157),
the amino acid sequence of the light-chain CDR1: QNINNE (SEQ ID NO: 158),
the amino acid sequence of the light-chain CDR2: DAS, and
the amino acid sequence of the light-chain CDR3: QSTYYDGNYVYA (SEQ ID NO: 156),
(b) the single-chain antibody having the amino acid sequence of the heavy-chain CDR3: GSYYDSHGYAYVSLW (SEQ ID NO: 149);
wherein the single-chain antibody (b) further comprises
the amino acid sequence of the heavy-chain CDR1: SGFSLSRYA (SEQ ID NO: 159),
the amino acid sequence of the heavy-chain CDR2: IGSGGST (SEQ ID NO: 160),
the amino acid sequence of the light-chain CDR1: QSISTA (SEQ ID NO: 161),
the amino acid sequence of the light-chain CDR2: SAS, and
the amino acid sequence of the light-chain CDR3: QSYYGSSSDNA (SEQ ID NO: 162);
(c) the single-chain antibody having
the amino acid sequence of the heavy-chain CDR3: ATDYGIYGYAYGHLW (SEQ ID NO: 150);
wherein the single-chain antibody (c) further comprises:
the amino acid sequence of the heavy-chain CDR1: SGIDLSSYA (SEQ ID NO: 163),
the amino acid sequence of the heavy-chain CDR2: IGSGGGT (SEQ ID NO: 164),
the amino acid sequence of the light-chain CDR1: QSISTA (SEQ ID NO: 161),
the amino acid sequence of the light-chain CDR2: DAS, and
the amino acid sequence of the light-chain CDR3: QTYFGSDTDNA (SEQ ID NO: 165);
(d) the single-chain antibody having
the amino acid sequence of the heavy-chain CDR3: ARYSGDNGGALNLW (SEQ ID NO: 151);
wherein the single-chain antibody (d) further comprises:
the amino acid sequence of the heavy-chain CDR1: SGFSLSSYA (SEQ ID NO: 166),
the amino acid sequence of the heavy-chain CDR2: ISSSGST (SEQ ID NO: 167),
the amino acid sequence of the light-chain CDR1: QHIRSY (SEQ ID NO: 168),
the amino acid sequence of the light-chain CDR2: AAS, and
the amino acid sequence of the light-chain CDR3: QRYYDIRNYGNG (SEQ ID NO: 169), and
(e) the single-chain antibody having
the amino acid sequence of the heavy-chain CDR3: ARYSGDNGGTLNLW (SEQ ID NO: 152);
wherein the single-chain antibody (e) further comprises:
the amino acid sequence of the heavy-chain CDR1: SGIDLRRYA (SEQ ID NO: 170),
the amino acid sequence of the heavy-chain CDR2: IASGNTD (SEQ ID NO: 171),
the amino acid sequence of the light-chain CDR1: QSISSY (SEQ ID NO: 172),
the amino acid sequence of the light-chain CDR2: AAS, and
the amino acid sequence of the light-chain CDR3: QSYYSISSYGNT (SEQ ID NO: 173).
6. A method for separating a human serum-derived IgG polyclonal antibody from a mixed liquid of two or more kinds of substances, said mixed liquid comprising human serum-derived IgG polyclonal antibody, said method comprising the steps of: contacting said mixed liquid with a separation agent; and separating a human serum-derived IgG polyclonal antibody from said mixed liquid, the separation agent comprising: a carrier; and a single-chain antibody which has a dissociation constant for a human serum-derived IgG polyclonal antibody of not more than 3.0×10−8 M and which binds to the surface of the carrier via a chemical bond,
wherein the single-chain antibody is selected from the following single-chain antibodies (a) to (e):
(a) the single-chain antibody having the amino acid sequence of the heavy-chain CDR3: ATRYDSYGYAYNYWFGTLW (SEQ ID NO: 148);
wherein the single-chain antibody (a) further comprises the following amino acid sequence (a-1) or (a-2):
(a-1) the amino acid sequence of the heavy-chain CDR1: SGIDLSSNA (SEQ ID NO: 153),
the amino acid sequence of the heavy-chain CDR2: ISTVGKT (SEQ ID NO: 154),
the amino acid sequence of the light-chain CDR1: ENINSE (SEQ ID NO: 155),
the amino acid sequence of the light-chain CDR2: DAS, and
the amino acid sequence of the light-chain CDR3: QSTYYDGNYVYA (SEQ ID NO: 156); and
(a-2) the amino acid sequence of the heavy-chain CDR1: SGIDLSSNA (SEQ ID NO: 153),
the amino acid sequence of the heavy-chain CDR2: ISTGGST (SEQ ID NO: 157),
the amino acid sequence of the light-chain CDR1: QNINNE (SEQ ID NO: 158),
the amino acid sequence of the light-chain CDR2: DAS, and
the amino acid sequence of the light-chain CDR3: QSTYYDGNYVYA (SEQ ID NO: 156),
(b) the single-chain antibody having the amino acid sequence of the heavy-chain CDR3: GSYYDSHGYAYVSLW (SEQ ID NO: 149);
wherein the single-chain antibody (b) further comprises
the amino acid sequence of the heavy-chain CDR1: SGFSLSRYA (SEQ ID NO: 159),
the amino acid sequence of the heavy-chain CDR2: IGSGGST (SEQ ID NO: 160),
the amino acid sequence of the light-chain CDR1: QSISTA (SEQ ID NO: 161),
the amino acid sequence of the light-chain CDR2: SAS, and
the amino acid sequence of the light-chain CDR3: QSYYGSSSDNA (SEQ ID NO: 162);
(c) the single-chain antibody having
the amino acid sequence of the heavy-chain CDR3: ATDYGIYGYAYGHLW (SEQ ID NO: 150);
wherein the single-chain antibody (c) further comprises:
the amino acid sequence of the heavy-chain CDR1: SGIDLSSYA (SEQ ID NO: 163),
the amino acid sequence of the heavy-chain CDR2: IGSGGGT (SEQ ID NO: 164),
the amino acid sequence of the light-chain CDR1: QSISTA (SEQ ID NO: 161),
the amino acid sequence of the light-chain CDR2: DAS, and
the amino acid sequence of the light-chain CDR3: QTYFGSDTDNA (SEQ ID NO: 165);
(d) the single-chain antibody having
the amino acid sequence of the heavy-chain CDR3: ARYSGDNGGALNLW (SEQ ID NO: 151);
wherein the single-chain antibody (d) further comprises:
the amino acid sequence of the heavy-chain CDR1: SGFSLSSYA (SEQ ID NO: 166),
the amino acid sequence of the heavy-chain CDR2: ISSSGST (SEQ ID NO: 167),
the amino acid sequence of the light-chain CDR1: QHIRSY (SEQ ID NO: 168),
the amino acid sequence of the light-chain CDR2: AAS, and
the amino acid sequence of the light-chain CDR3: QRYYDIRNYGNG (SEQ ID NO: 169), and
(e) the single-chain antibody having
the amino acid sequence of the heavy-chain CDR3: ARYSGDNGGTLNLW (SEQ ID NO: 152);
wherein the single-chain antibody (e) further comprises:
the amino acid sequence of the heavy-chain CDR1: SGIDLRRYA (SEQ ID NO: 170),
the amino acid sequence of the heavy-chain CDR2: IASGNTD (SEQ ID NO: 171),
the amino acid sequence of the light-chain CDR1: QSISSY (SEQ ID NO: 172),
the amino acid sequence of the light-chain CDR2: AAS, and
the amino acid sequence of the light-chain CDR3: QSYYSISSYGNT (SEQ ID NO: 173).
2. The separation agent according to
3. The separation agent according to
4. The separation agent according to
5. The separation agent according to
7. The method according to
8. The method according to
9. The method according to
10. The method according to
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This application includes an electronically submitted sequence listing in .txt format. The .txt file contains a sequence listing entitled “2021-04-17_1261-0209PUS1_ST25.txt” created on Apr. 17, 2021, and is 16,673 bytes in size. The sequence listing contained in this .txt file is part of the specification and is hereby incorporated by reference herein in its entirety.
The present invention relates to a method for screening a single-chain antibody and a single-chain antibody.
Various forms of molecular targeted drugs have been studied and developed, including antibody drugs and low molecular weight drugs, as well as peptide drugs, in vivo protein preparations such as cytokines, siRNAs and aptamers (see Patent Document 1, for example). The use of antibodies as therapeutic agents are useful, because of their specificities, in the treatment of pathological conditions in which diseased cells express specific antigens. Antibodies bind to proteins expressed on the cell surface as antigens, and effectively act on the cells to which they are bound. Antibodies are characterized by having a long half-life in blood and high specificity for antigens, and are extremely useful also as antitumor drugs.
To obtain such an antibody, a technique is known in which an antibody is obtained by panning (referred to as “panning” by making an analogy to “washing out gold dust from the pebbles”) using an antibody library. For example, a method is known in which the variable region of a human antibody is expressed as a single-chain antibody (scFv) on phage surface by the phage display method, and a phage which binds to an antigen is selected. By analyzing the gene of the selected phage, it is possible to determine the DNA sequence encoding the variable region of the human antibody which binds to the antigen. Once the DNA sequence of the scFv which binds to the antigen is determined, a suitable expression vector containing the sequence can be prepared to easily produce the human antibody (see Patent Documents 2 and 3, for example).
As described above, a method for obtaining an antibody as a candidate for an antibody drug by panning using an antibody library, and the like are known. However, such a method requires a blocking operation, since an antigen is usually immobilized on a tube or plate made of polystyrene when allowing phages to bind to the antigen, in the technical field, and in addition, there are cases where a protein adsorbed on the tube and the like may be denatured. As a result, some of the phages in a phage library bind to a protein used for blocking, or bind the denatured protein, resulting in a problem that phages which bind to antigens other than the antigen of interest are obtained.
On the other hand, in contrast to the above described method for obtaining an antibody, a method has been developed in which multilamellar liposomes are used to obtain a peptide which binds to a specific antibody from a peptide library (Non-patent Document 1). In Non-patent Document 1, it has been confirmed that, when a library of peptides which are expressed on the surface of phages by the phage display method is applied for an anti-octapeptide (FVNQHLCK, SEQ ID NO: 35) antibody immobilized on multilamellar liposomes, as a model, the octapeptide (FVNQHLCK, SEQ ID NO: 35) can be selectively obtained.
An object of the present invention is to provide a method for screening a single-chain antibody having a high separation efficiency and an extremely high antigen-binding capacity, as well as a single-chain antibody obtained by the screening method.
The present inventors have found out that, in the case of obtaining an antibody of interest by panning using an antibody library prepared by the phage display method, it is possible to solve the problem that phages which bind to antigens other than the antigen of interest are likely to be obtained, which is a problem associated with the use of a conventional method in which an antigen is immobilized on a tube or the like, by the use of a method in which an antigen is coupled to multilamellar liposomes. The present invention is as follows.
[1] A method for screening a single-chain antibody which binds to an antigen, the method including the steps of:
[2] The method according to [1], wherein the single-chain antibody is derived from a rabbit.
[3] The method according to [1] or [2], wherein the antigen is a protein.
[4] The method according to [3], wherein the protein is an antibody.
[5] The method according to [4], wherein the antibody is a human serum-derived IgG polyclonal antibody or a human serum-derived IgA polyclonal antibody.
[6] The method according to [4] or [5], wherein the single-chain antibody is a single-chain antibody which binds to the L chain of a human-derived antibody.
[7] A method for producing an antibody, the method including the steps of:
[8] The method according to [7], wherein the DNA sequence encoding the antibody encodes a humanized antibody.
[9] A single-chain antibody having a dissociation constant for a human serum-derived IgG polyclonal antibody of not more than 3.0×10−8 M.
[10] The single-chain antibody according to [9], which also binds to a human serum-derived IgA polyclonal antibody.
[11] A single-chain antibody having a dissociation rate constant for a human serum-derived IgA polyclonal antibody of not more than 1.0×10−3 s−1.
[12] A single-chain antibody having a dissociation rate constant for the L chain of a human-derived antibody of not more than 1.0×10−3 s−1.
According to the present invention, it is possible to provide a method for screening a single-chain antibody having a high separation efficiency and an extremely high antigen-binding capacity, as well as a single-chain antibody obtained by the screening method.
Since multilamellar liposomes have a good dispersibility, the method using multilamellar liposomes allows for efficiently bringing an antibody with an antigen coupled to the multilamellar liposomes as compared to a conventional method, and it also allows for easy recovery of the antibody by centrifugation. Further, the use of multilamellar liposomes enables to reduce phages which are non-specifically adsorbed on a carrier, to an extremely low level. In addition, since the antigen can laterally diffuse on the membrane surface of the multilamellar liposomes, the antigen exhibits a high binding capacity with phages in a library. Accordingly, the present method allows for obtaining a single-chain antibody having a high separation efficiency and an extremely high antigen-binding capacity.
The present invention includes a first invention relating to a method for screening a single-chain antibody, and a second invention relating to a single-chain antibody. In the present specification, multilamellar liposomes are sometimes referred to as MLVs (multilamellar liposome vesicles). Further, single-chain antibodies are sometimes referred to as scFvs (single chain Fvs). The single-chain antibodies (scFvs) in the present invention are sometimes referred to as “single chain Fvs” or the like in the technical filed, as one type of low molecular weight antibodies.
The following description includes a description regarding the use of a rabbit-derived single-chain antibody as the single-chain antibody in the present invention. However, such a description is merely an example of the case where the single-chain antibody used is derived from a rabbit, and the single-chain antibody to be used in the present invention is not limited to a rabbit-derived single-chain antibody.
<1. First Invention>
The first invention of the present invention includes the following first and second embodiments.
The first embodiment: a method for screening a single-chain antibody which binds to an antigen, the method including the steps of: preparing an antigen coupled to multilamellar liposomes; preparing a phage library presenting single-chain antibodies; and selecting a phage presenting the single-chain antibody which binds to the antigen coupled to multilamellar liposomes; from the phage library.
The second embodiment: a method for producing an antibody, the method including the steps of: performing screening by the screening method according the first embodiment; determining the amino acid sequence of the screened single-chain antibody; preparing a DNA sequence encoding the antibody based on the sequence of the variable region of the determined amino acid sequence; expressing the prepared DNA sequence in a host cell.
The first embodiment in the first invention of the present invention is a method for screening a single-chain antibody which binds to an antigen, the method including the steps of: preparing an antigen coupled to multilamellar liposomes; preparing a phage library presenting single-chain antibodies; and selecting a phage presenting the single-chain antibody which binds to the antigen coupled to multilamellar liposomes; from the phage library.
The present screening method may be a method for screening a candidate for a single-chain antibody which binds to the above described antigen.
<(1) Step of Preparing Antigen Coupled to Multilamellar Liposomes>
[Multilamellar Liposomes (MLVs)]
Multilamellar liposomes are not particularly limited as long as an antigen can be coupled thereto. For example, multilamellar liposomes can be prepared by a known method such as the method described in Journal of Biotechnology 131 (2007) 144-149. Specifically, multilamellar liposomes can be prepared, for example, by hydrating appropriate amounts of dipalmitoylphosphatidylcholine (DPPC), dicetyl phosphate (DCP), and N-(4-(p-maleimidophenyl)butyryl)dipalmitoylphosphatidylethanolamine (MPB-DPPE).
At this time, multilamellar liposomes and unilamellar liposomes are often obtained in a mixed state, by performing hydration alone. Thus, multilamellar liposomes are preferably separated by centrifugation before use. The conditions of centrifugation are not particularly limited as long as the multilamellar liposomes can be separated. The centrifugation may be carried out, for example at 25° C. for two minutes, at 20,000 g.
[Antigen]
The antigen to be used is not particularly limited as long as it is a substance to which a single-chain antibody to be screened by the screening method according to the present embodiment binds. Examples thereof include cells, proteins, lipids, and sugar chains. Among these, a protein is preferred, and among proteins, an antibody is preferred. The antigen can be selected as appropriate depending on the application of the single-chain antibody to be obtained.
The biological species of the antibody to be used as an antigen is not particularly limited, and can be selected as appropriate depending on the application of the single-chain antibody to be obtained. Examples thereof include humans, rats, mice, rabbits, chickens, goats, sheep, cows, horses, dogs, cats, and monkeys. Preferred are humans, rats, mice, rabbits, chickens, and goats. The antibody to be used as an antigen may be a monoclonal antibody or a polyclonal antibody, and it can be selected as appropriate depending on the application of the single-chain antibody to be obtained.
Further, the antibody to be used as an antigen may be one type or two or more types selected from the group consisting of IgG, IgM, IgA, IgD and IgE antibodies. Further, an antibody belonging to a subclass of each type of antibody may also be used, and one type or two or more types of such subclass antibodies may be used.
In cases where the antibody to be used as an antigen is a human IgG antibody, examples of its subclass antibody include a human IgG1 antibody, a human IgG2 antibody, a human IgG3 antibody, and a human IgG4 antibody. Any one type, two or more types, three or more types, or all four types of these antibodies may be used.
In cases where the antibody to be used as an antigen is a human serum-derived IgG polyclonal antibody, examples of its subclass antibody include a human serum-derived IgG1 polyclonal antibody, a human serum-derived IgG2 polyclonal antibody, a human serum-derived IgG3 polyclonal antibody, and a human serum-derived IgG4 polyclonal antibody. Any one type, two or more types, three or more types, or all four types of these antibodies may be used.
Further, if a single-chain antibody selected by the present screening method binds to an antigen coupled to multilamellar liposomes, and does not bind to other antigens, the single-chain antibody can be used as a highly specific single-chain antibody. On the other hand, a single-chain antibody selected by the present screening method has a possibility of binding to an antigen coupled to multilamellar liposomes, as well as to other antigens. Such a single-chain antibody can be used as a single-chain antibody which binds to a common region of two or more different antigens, or as a single-chain antibody which binds to two or more different sites in the same amino acid sequence. Any of these single-chain antibodies can be selected and used depending on the application, and any of these are preferred embodiment(s).
The single-chain antibody which binds to a common region of two or more different antigens can be determined, for example, by performing screenings for two or more different antigens, individually, and then comparing the amino acid sequences of the single-chain antibodies selected by the respective screenings. This can be easily understood by those skilled in the art.
Further, the single-chain antibody which binds to two or more different sites in the same amino acid sequence can be determined, for example, by confirming the binding capacity of the single-chain antibody which has been selected by a screening using a certain antigen, for other antigens. This can be easily understood by those skilled in the art.
Examples of the single-chain antibody which binds to a common region of two or more different antibodies include a single-chain antibody which binds to a common region included in the light chains (L chains), specifically, the lambda chains or the kappa chains, of two or more different antibodies. In particular, since the amino acid sequence of the lambda chain or the kappa chain does not vary depending on the isotype, if a single-chain antibody which binds to an amino acid sequence contained in the lambda chain or the kappa chain is selected, the selected single-chain antibody recognizes and binds to the amino acid sequence regardless of the isotype. This can be easily understood by those skilled in the art.
Those skilled in the art can confirm that the selected single-chain antibody binds to an amino acid sequence contained in the light chain (L chain) of an antibody, specifically, that it binds to an amino acid sequence contained in the lambda chain or the kappa chain, for example, by a known method such as Western blotting.
There is no particular limitation on the antibody to be used as an antigen for selecting a single-chain antibody which binds to an amino acid sequence contained in the light chain (L chain) regardless of the isotype. However, preferred is an IgA antibody, such as, for example, a human serum-derived IgA polyclonal antibody.
The reason for this is as follows. In view of the fact that IgA antibodies do not have a complement activity while IgG antibodies and IgM antibodies have a complement activity, for example, IgA antibodies, rather than IgM antibodies, are thought to have functions and structures significantly different from those of the IgG antibodies, when considered based on IgG antibodies. Accordingly, the use of an IgA antibody, rather than the use of an IgM antibody, for example, facilitates the selection of a single-chain antibody which binds to an amino acid sequence contained in the light chain (L chain).
Further, it is also because, IgA antibodies forming monomers or dimers have a lower molecular weight as compared to IgM antibodies forming pentamers, for example, and have a higher dispersibility on multilamellar liposomes, and accordingly, the use of an IgA antibody, rather than the use of an IgM antibody, results in a higher screening efficiency.
In addition, IgA antibodies can be used as antibody drugs which have a high therapeutic effect in the mucous membrane.
[Step of Coupling Antigen to Multilamellar Liposomes]
Coupling of an antigen to multilamellar liposomes can be performed by any method without particular limitation, as long as the coupled antigen is not liberated form the multilamellar liposomes. For example, the coupling can be carried out by a known method such as the method disclosed in Non-patent Document 1. Specific examples of the method include one in which an excessive amount of 2-iminothiolane hydrochloride, in molar ratio, is added to a mixed liquid of an antigen and multilamellar liposomes, and a reaction is allowed to proceed while stirring. The coupling may be carried out, for example, by adding to the mixed liquid of an antigen and multilamellar liposomes, 2-iminothiolane hydrochloride in amount 10 times the amount of the antigen, in molar ratio, and allowing a reaction to proceed at 25° C. for three hours or more, while stirring.
<(2) Step of Preparing Phage Library Presenting Single-Chain Antibodies>
[Phage Library Presenting Single-Chain Antibodies]
The phage library to be prepared is not particularly limited as long as it is a library of phages presenting single-chain antibodies, and a known library or a commercially available library may be used. There is no particular limitation on the animal from which a single-chain antibody is derived. However, the single-chain antibody preferably has a high antigen-binding capacity, and is derived from an animal, such as, for example, a human, a rat, a mouse, a rabbit, a chicken, a goat, a sheep, a cow, a horse, a dog, a cat, or a monkey. The single-chain antibody is more preferably derived from an animal, such as, for example, a human, a rat, a mouse, a rabbit, a chicken, or a goat, still more preferably derived from a mouse or a rabbit, and particularly preferably derived from a rabbit.
The construction of a phage library can be carried out by a known method, such as the method disclosed in Japanese Patent Application No. 2013-233096.
In the case of using an immunized animal, the construction of a phage library can be carried out, for example, as follows. A specific antigen is administered to an animal to be immunized, and the total RNA is obtained from the spleen of the thus immunized animal, and then a cDNA library is constructed by reverse transcription polymerase chain reaction (RT-PCR). Subsequently, specific primers are used to amplify the gene of the variable region (VH domain) of the heavy chain (H chain), and the gene of the variable region (VL domain) of the light chain (L chain), by PCR.
There is no particular limitation on the primers to be used in cases where a rabbit is used as the immunized animal, as long as the primers allow for specifically amplifying the genes of interest by PCR. Examples of sense primers to be used for amplifying the gene of the variable region (VH domain) of the heavy chain (H chain) include:
Examples of antisense primers to be used include:
Examples of sense primers to be used for amplifying the gene of the variable region (VL domain) of the light chain (L chain) include:
Examples of antisense primers to be used include:
Note that, in the above described sequences, W represents A or T, R represents A or G, M represents A or C, K represents T or G, Y represents T or C, S represents G or C, H represents A, C or T, B represents G, C or T, V represents A, G or C, D represents A, G or T, and N represents A, G, C or T, based on the IUPAC nomenclature of bases.
Next, the thus produced PCR products are subjected to a treatment by specific restriction enzymes, and the like, so that they can be inserted into a phagemid vector. Further, the phagemid vector to be used is also subjected to a treatment by specific restriction enzymes, and the like. Subsequently, each of the genes treated by the restriction enzymes are inserted into the phagemid vector treated by the restriction enzymes.
In this manner, a recombinant phagemid vector into which the gene of the variable region (VH domain) of the heavy chain (H chain), and the gene of the variable region (VL domain) of the light chain (L chain) are inserted, is introduced into host cells, such as, for example, cells of Escherichia coli. The transfected host cells are further infected with a helper phage, followed by culturing, to obtain a library of phages presenting rabbit-derived single-chain antibodies, in the resulting culture supernatant. The type of the helper phage to be used above is not particularly limited, and examples thereof include VCSM13.
<(3) Step of Selecting Phage Presenting Single-Chain Antibody which Binds to Antigen Coupled to Multilamellar Liposomes from Phage Library (Selection Step)>
The present step (selection step) includes: a step of allowing the antigen to bind to the single-chain antibodies expressed on the surface of phages in the phage library (binding step); a step of removing phages presenting single-chain antibodies which did not bind to the antigen coupled to multilamellar liposomes, by washing (washing step); and a step of dissociating (eluting) the phage presenting the single-chain antibody bound to the antigen coupled to multilamellar liposomes, from the antigen (elution step).
<(3-1) Binding Step>
The present step is a step of allowing the antigen to bind to the single-chain antibodies expressed on the surface of phages in the phage library. The method for carrying out the binding step is not particularly limited, as long as the method allows for sufficient binding between the antigen and the single-chain antibodies. The binding step can be carried out, for example, under the following conditions.
(Quantitative Ratio of Antigen and Phage Library)
The quantitative ratio of the antigen and the phages in the library is not particularly limited, as long as the ratio allows for a sufficient binding between the two. The quantitative ratio of the number of total phages in the library vs the number of antigen molecules is usually 1:5 or more, preferably 1:100 or more, and more preferably 1:1000 or more. When the quantitative ratio is within the above range, the number of antigen molecules will be sufficient relative to the number of the single-chain antibodies expressed on the phage surface, and a sufficient binding between the antigen and the single-chain antibodies can be expected.
(Solvent)
The type of the solvent to be used when allowing the antigen to bind to the single-chain antibodies expressed on the surface of phages in the phage library is not particularly limited, as long as the solvent allows for a sufficient binding between the two. For example, it is possible to use a solvent commonly used in the field, such as phosphate buffered saline (PBS).
(Temperature)
The temperature for allowing the antigen to bind to the single-chain antibodies expressed on the surface of phages in the phage library is not particularly limited, as long as the temperature allows for a sufficient binding between the two. However, in order to avoid degradation, denaturation and the like, the binding is preferably carried out at, for example, at room temperature, such as 25° C., and more preferably at a low temperature, such as 4° C.
(Period of Time)
The period of time for allowing the antigen to bind to the single-chain antibodies expressed on the surface of phages in the phage library is not particularly limited, as long as it allows for a sufficient binding between the two. However, the binding is carried out, for example, for 30 minutes or more, preferably one hour or more, and still more preferably overnight.
(Other Matters)
The binding reaction of the antigen and the single-chain antibodies expressed on the surface of phages in the phage library is preferably carried out, for example, while rotating, so that the antigen molecules and the phages can be sufficiently stirred during the reaction. Further, a reaction vessel such as a tube to be used for binding the antigen and the single-chain antibodies is preferably subjected to blocking, in advance. Examples of blocking agents include known blocking agents, such as those supplemented with bovine serum albumin (BSA). In addition, such a blocking agent can be added to the solvent to be used for the binding reaction, in advance.
<(3-2) Washing Step>
The present step is a step of removing phages presenting single-chain antibodies which did not bind to the antigen coupled to multilamellar liposomes, by washing. The method for carrying out the washing step is not particularly limited, as long as the phages presenting single-chain antibodies which did not bind to the antigen can be removed by washing. The washing step can be carried out, for example, under the following conditions.
(Centrifugation and Solvent Replacement)
After the binding reaction of the antigen and the single-chain antibodies expressed on the surface of phages in the phage library, the phages bound to the antigen coupled to multilamellar liposomes are precipitated by centrifugation, and the phages which did not bind to the antigen are contained in the supernatant. Therefore, the phages bound to the antigen coupled to multilamellar liposomes can be selectively obtained, by removing the supernatant, and then adding a solvent to the pellets to prepare a suspension.
The solvent to be used at this time is not particularly limited. However, the solvent is preferably the same as that used in the above described “(3-1) Binding Step”, and PBS or the like can be used, for example. Further, a blocking agent such as BSA can be added to the solvent, in advance. Further, in cases where the suspension obtained by adding such a solvent to the pellets is transferred to a vessel such as a fresh tube, it is preferred that the vessel be also subjected to blocking in advance. Further, such a blocking agent can be added to the solvent to be used for the binding reaction, in advance.
The conditions of centrifugation is not particularly limited, as long as the phages bound to the antigen coupled to multilamellar liposomes can be separated from the phages which did not bind to the antigen. The centrifugation may be carried out, for example, at 4° C. for two minutes, at 20,000 g. The centrifugation and solvent replacement may be carried out once, or repeated a plurality of times. However, the centrifugation and solvent replacement are usually repeated twice or more, and preferably repeated three times or more.
<(3-3) Elution Step>
The present step is a step of dissociating (eluting) the phage presenting the single-chain antibody bound to the antigen coupled to multilamellar liposomes, from the antigen. The method for carrying out the elution step is not particularly limited. The elution step can be carried out, for example, according to a known method such as the method disclosed in Non-patent Document 1.
As a solution to be used for eluting the phages, a glycine-hydrochloric acid buffer solution or the like can be used, for example. Further, after eluting the phages, the resulting solution may be neutralized, and a tris-hydrochloric acid buffer solution or the like, for example, can be used for the neutralization.
<(3-4) Optional Steps>
The present selection step may include optional steps, as appropriate, in addition to the above described three steps (the binding step, the washing step, and the elution step). Examples of the optional steps include: a step of amplifying the selected phage (amplification step); a step of repeating the above described selection step (repetition step); a step of determining the gene sequence of the selected phage (gene sequencing step); a step of selecting a clone based on the sequence determined in the gene sequencing step (clone selection step), and a step of evaluating the binding activity for the antigen of the single-chain antibody presented by the selected phage (antigen-binding activity evaluation step).
[Amplification Step]
The present step is a step of amplifying the phage selected in the selection step. The method for carrying out the amplification step is not particularly limited. The amplification step can be carried out, for example, under the following conditions.
(Infection of Host Cells with Phage, and Culture of Host Cells Infected with Phage)
The phage selected in the selection step can be amplified by infecting host cells with the phage. The method therefor is not particularly limited, and the infection and amplification can be achieved, for example, according to a known method such as the method disclosed in Non-patent Document 1. The host cells to be used are not particularly limited, as long as the phage can be grown. The host cells may be, for example, Escherichia coli cells, and strains such as TG1 strain or XL-1 Blue strain may be used, for example. Further, it is preferred that the host cells be cultured in advance, and those in the middle stage of the exponential growth be used. The conditions for culturing the host cells which have been infected with the phage are not particularly limited, and the host cells may be cultured, for example, at 37° C. with shaking at 200 rpm.
(Infection of Host Cells with Helper Phage and Production of Phages in Culture Supernatant)
By infecting the host cells which have been infected with the phage, further with a helper phage, and then culturing the infected host cells, it is possible to allow the secretion of the phage presenting the single-chain antibody, and the single-chain antibody, in the culture supernatant. The method therefor is not particularly limited, and the secretion of the phage and the single-chain antibody can be achieved for example, according to a known method such as the method disclosed in Non-patent Document 1. The helper phage to be used at this time is not particularly limited, and examples thereof include VCSM13. Further, the culture conditions are not particularly limited, and the cells may be cultured, for example, at 37° C. with shaking at 200 rpm.
[Repetition Step]
The above described selection step may be repeated, using a library of the phages selected in the above described selection step, or a library of the phages amplified in the above described amplification step.
By repeating one “round”, which consists of the above described selection step, it is possible to further select a phage having a higher binding capacity for the antigen. The number of rounds is not particularly limited. A larger number of rounds leads to obtaining a phage having an extremely high binding capacity for the antigen; whereas a smaller number of rounds enables a quick and efficient screening, and thus is useful. The present method is useful in that it allows for obtaining a phage having an extremely high binding capacity for the antigen, with a smaller number of rounds as compared to a conventional technique.
The number of times for carrying out the repetition step is usually three times or less, preferably twice or less, more preferably once or less, and still more preferably 0 times. When the number of times for carrying out the repetition step is 0 times, it means that the selection step is carried out only once.
[Gene Sequencing Step]
The present step is a step of determining the gene sequence of the variable region (VH domain) of the heavy chain (H chain) and the gene sequence of the variable region (VL domain) of the light chain (L chain) of each phage, using a library of the phages selected in the above described selection step. The present step may be carried out as the final round, and/or carried out between the rounds.
The method therefor is not particularly limited, and the gene sequences can be determined according to a known method such as the method disclosed in Non-patent Document 1. For example, the gene sequences can be determined, for example, by the following method.
By the method described in the section of “Infection of Host Cells with Phage, and Culture of Host Cells Infected with Phage” in the above described amplification step, Escherichia coli cells infected with the phages are allowed to form single colonies, and each colony is subcloned. Subsequently, the sequences of the gene of the variable region (VH domain) of the heavy chain (H chain), and the gene of the variable region (VL domain) of the light chain (L chain) can be analyzed and determined for each colony. The gene sequences can be analyzed using a known technique. If the gene sequences can be determined, the amino acid sequences encoded by the gene sequences can also be determined. When the gene sequences are determined in this manner, it is also possible to monitor the efficiency of screening.
[Clone Selection Step]
The present step is a step of selecting a clone, based on each sequence determined in the gene sequencing step. This step is a step of selecting a clone of host cells infected with the phage containing a desired gene sequence of the variable region (VH domain) of the heavy chain (H chain) and a desired gene sequence of the (VL domain) of the light chain (L chain). This step is also effective for eliminating overlapping clones.
The present step may be carried out as the final round, and/or carried out between the rounds. If such a clone can be selected, it is possible to select a host cell infected with a phage having a higher binding capacity for the antigen, thereby allowing for a more efficient screening.
[Antigen-Binding Activity Evaluation Step]
The present step is a step of evaluating the binding activity for the antigen of the antibody presented by the selected phage. The method therefor is not limited, as long as the binding activity for the antigen of the antibody presented by the phage can be evaluated.
The evaluation can be carried out, for example, by the method to be described in Example 3-2. Specifically, host cells containing a phagemid are allowed to form a single colony, and the supernatant obtained after cell lysis is applied on a plate on which an antigen is immobilized. Subsequently, the absorbance is measured using a microplate reader.
The present step may be carried out as the final round, and/or carried out between the rounds. If a clone containing the gene of the antibody having a high binding capacity for the antigen can be selected, a more efficient screening can be carried out using the clone.
In addition, the dissociation rate constant koff or the dissociation constant KD measured using a Biacore, or the like, as will be described in Example 4 and Example 6, can be used as an index.
The method for preparing a sample to be used in the measurement of the dissociation rate constant koff or the dissociation constant KD is not particularly limited. For example, as will be shown in Examples, cells obtained from a colony of phagemid-containing host cells are cultured, followed by cell lysis, and the supernatant obtained after centrifugation can be used as a sample.
In addition, whether the phage and the single-chain antibody have been secreted from the host cells, or whether they are present within the periplasm, can be confirmed as follows. For example, as will be shown in Examples, when a DNA fragment containing the gene of the single-chain antibody is amplified using a phagemid vector, and the amplified fragment is inserted into an appropriate vector, such as a pET22 vector (manufactured by Merck KGaA), the single-chain antibody will be expressed in the form in which a pelB leader signal sequence is fused to the N-terminus, and a histidine tag (6×His-tag) is fused to the C-terminus. After culturing the host cells containing the above described recombinant vector, it is possible to obtain the culture supernatant, and the intracellular soluble fraction from the cells, by an appropriate method. The thus obtained culture supernatant and the intracellular soluble fraction are each eluted using a column capable of trapping a histidine tag, or the like, and the dissociation constant KD can be measured using the resulting eluants.
The dissociation rate constant koff and the dissociation constant KD will be described below.
[Dissociation Rate Constant koff]
In the present specification, the dissociation rate constant koff for the binding of the single-chain antibody to the antigen is defined as follows. The dissociation rate constant koff is usually not more than 3.0×10−3 s−1, preferably not more than 1.0×10−3 s−1, more preferably not more than 4.0×10−4 s−1, still more preferably not more than 2.0×10−4 s−1, further still more preferably not more than 5.0×10−5 s−1, particularly preferably not more than 4.0×10−5 s−1, and more particularly preferably not more than 3.0×10−5 s−1. A lower dissociation rate constant koff indicates a higher binding capacity for the antigen, and thus, a higher usefulness as an antibody.
In cases where an antigen is represented as Ag, the concentration of the antigen as [Ag], an antibody as Ab, the concentration of the antibody as [Ab], an antigen-antibody complex as Ag·Ab, the concentration of the antigen-antibody complex as [Ag·Ab], a binding rate constant as kon, and the dissociation rate constant as koff, the binding reaction between the antigen and the single-chain antibody is represented by the following equations (1) and (2):
These equations can be converted to the following equation (3):
In a liquid delivery system such as Biacore, the value of [Ab] is 0 at the time of washing the sensor chip, and thus, the above described equation (3) is represented as the following equation (4):
Further, when the [Ag·Ab] at the time t=0 is represented as [Ag·Ab]0, it can be represented as the following equation (5):
In the case of calculating the dissociation rate constant for the binding of the single-chain antibody to the antigen, using a liquid delivery system such as Biacore, the dissociation rate constant can be obtained by: drawing a measurement graph, in which the time: t is plotted on the horizontal axis, and
is plotted on the vertical axis; and calculating the dissociation rate constant from the slope of the graph.
(Method for Measuring Dissociation Rate Constant koff)
The method for measuring the dissociation rate constant is not particularly limited, and the measurement can be carried out, for example, using a known apparatus such as BiacoreX-100 (manufactured by GE Healthcare Inc.) as a measuring apparatus, and by drawing a measurement graph as described above and calculating the dissociation rate constant from the slope of the graph.
[Dissociation Constant KD]
The dissociation constant KD is usually not more than 3.0×10−8 M, preferably not more than 1.0×10−8 M, more preferably not more than 6.0×10−9 M, still more preferably not more than 1.0×10−9 M, further still more preferably not more than 6.0×10−10 M, and particularly preferably not more than 1.0×10−10 M. A lower dissociation constant indicates a higher binding capacity for the antigen, and thus, a higher usefulness as an antibody. Note that a common antibody has a KD of about 10 nM, whereas the single-chain antibody in the present embodiment has a KD within the above described range. This indicates that the single-chain antibody has a markedly higher binding capacity as compared to a common antibody.
(Method for Measuring Dissociation Constant KD)
The method for measuring the dissociation constant KD is not particularly limited, and a known method can be used. For example, Biacore X-100 (manufactured by GE Healthcare Inc.) can be used as a measuring apparatus.
[Complementarity Determining Regions (CDRs) of VH Chain of Single-Chain Antibody]
The complementarity determining regions (CDRs) of the VH chain of a single-chain antibody includes CDR1, CDR2, and CDR3. As is well known, the amino acid sequence of CDR3, among the above described CDRs, contributes the most to the binding capacity for an antigen.
The amino acid sequences of the CDRs of the VH chain of the single-chain antibody in the present embodiment are not particularly limited, as long as an antibody constructed using the CDR sequences binds to an antigen. Of the amino acid sequences of the CDRs, the amino acid sequence of CDR3 is preferably the amino acid sequence of CDR3 of any one of the VH chains described in Examples in the present specification, in cases where the present method is carried out using a human serum-derived IgG polyclonal antibody or a human serum-derived IgA polyclonal antibody as the antigen, and a rabbit-derived single-chain antibody as the single-chain antibody. This is because an antibody constructed using such a CDR3 sequence has a high binding capacity for the antigen. Further, among these sequences, more preferred is an amino acid sequence which allows an antibody constructed therewith to have a higher binding capacity for the antigen.
The same applies to the amino acid sequence of CDR1 and the amino acid sequence of CDR2. The amino acid sequences of CDR1 and CDR2 are preferably the amino acid sequences of CDR1 and CDR2, respectively, of any one of the VH chains described in Examples in the present specification, in cases where the present method is carried out using a human serum-derived IgG polyclonal antibody or a human serum-derived IgA polyclonal antibody as the antigen, and a rabbit-derived single-chain antibody as the single-chain antibody. This is because an antibody constructed using such CDR1 and CDR2 sequences has a high binding capacity for the antigen. Further, among these sequences, more preferred are amino acid sequences which allow an antibody constructed therewith to have a higher binding capacity for the antigen.
[Amino Acid Sequences Substantially Homologous to Amino Acid Sequences of CDRs of VH Chain]
Each of the amino acid sequences of CDR1, CDR2, and CDR3 of the VH chain in the present embodiment is not particularly limited, as long as an antibody constructed using the CDR sequences binds to an antigen. In cases where the present method is carried out using a human serum-derived IgG polyclonal antibody or a human serum-derived IgA polyclonal antibody as the antigen, and a rabbit-derived single-chain antibody as the single-chain antibody, the amino acid sequences of CDR1, CDR2, and CDR3 of the VH chain may be amino acid sequences having an identity of 80% or more, preferably 90% or more, and more preferably 95% or more to the amino acid sequences of CDR1, CDR2, and CDR3, respectively, of any one of the VH chains described in Examples in the present specification.
Further, in cases where the present method is carried out using a human serum-derived IgG polyclonal antibody or a human serum-derived IgA polyclonal antibody as the antigen, and a rabbit-derived single-chain antibody as the single-chain antibody, the CDR1, CDR2, and CDR3 of the VH chain may have the same amino acid sequences as the amino acid sequences of CDR1, CDR2, and CDR3, respectively, of any one of the VH chains described in Examples in the present specification, except that one to several amino acids are substituted, deleted, inserted and/or added. The expression “one to several” as used herein refers preferably to a number from 1 to 5, and more preferably from 1 to 3.
The above described substitution is preferably a conservative substitution, and a conservative mutation is a mutation in which substitution takes place mutually among Phe, Trp, and Tyr, if the substitution site is an aromatic amino acid; among Leu, Ile, and Val, if the substitution site is a hydrophobic amino acid; between Gln and Asn, if the substitution site is a polar amino acid; among Lys, Arg, and His, if the substitution site is a basic amino acid; between Asp and Glu, if the substitution site is an acidic amino acid; and between Ser and Thr, if the substitution site is an amino acid having a hydroxyl group.
Examples of the conservative substitution include: substitution of Ala with Ser or Thr; substitution of Arg with Gln, His or Lys; substitution of Asn with Glu, Gln, Lys, His, or Asp; substitution of Asp with Asn, Glu or Gln; substitution of Cys with Ser or Ala; substitution of Gln with Asn, Glu, Lys, His, Asp, or Arg; substitution of Glu with Gly, Asn, Gln, Lys, or Asp; substitution of Gly with Pro; substitution of His with Asn, Lys, Gln, Arg, or Tyr; substitution of Ile with Leu, Met, Val, or Phe; substitution of Leu with Ile, Met, Val, or Phe; substitution of Lys with Asn, Glu, Gln, His, or Arg; substitution of Met with Ile, Leu, Val, or Phe; substitution of Phe with Trp, Tyr, Met, Ile, or Leu; substitution of Ser with Thr or Ala; substitution of Thr with Ser or Ala; substitution of Trp with Phe or Tyr; substitution of Tyr with His, Phe, or Trp; and substitution of Val with Met, Ile, or Leu.
The amino acid sequence(s) may be modified, as long as an antibody constructed using the modified sequence(s) binds to an antigen. Examples of the modification include amidation, addition of a lipid chain (aliphatic acylation (such as palmitoylation and myristoylation), prenylation (such as famesylation and geranylgeranylation) and the like), phosphorylation (phosphorylation on a serine residue, a threonine residue, a tyrosine residue, etc.), acetylation, and addition of a sugar chain (such as N-glycosylation and O-glycosylation).
[Complementarity Determining Regions (CDRs) of VL Chain of Single-Chain Antibody]
The complementarity determining regions (CDRs) of the VL chain of a single-chain antibody includes CDR1, CDR2, and CDR3. As is well known, the amino acid sequences of the CDRs of the VL chain also contribute to the binding capacity for an antigen.
The amino acid sequences of the CDRs of the VL chain of the single-chain antibody in the present embodiment are not particularly limited, as long as an antibody constructed using the CDR sequences binds to an antigen. The amino acid sequences of CDR1, CDR2, and CDR3 are preferably the amino acid sequences of CDR1, CDR2, and CDR3, respectively, of any one of the VL chains described in Examples in the present specification, in cases where the present method is carried out using a human serum-derived IgG polyclonal antibody or a human serum-derived IgA polyclonal antibody as the antigen, and a rabbit-derived single-chain antibody as the single-chain antibody. This is because an antibody constructed using such CDR sequences has a high binding capacity for the antigen. Further, among these sequences, more preferred are amino acid sequences which allow an antibody constructed therewith to have a higher binding capacity for the antigen.
[Amino Acid Sequences Substantially Homologous to Amino Acid Sequences of CDRs of VL Chain]
The description to be given here is the same as that given above in the section of “Amino Acid Sequences Substantially Homologous to Amino Acid Sequences of CDRs of VH Chain”.
[Framework Regions (FR) of VH Chain of Single-Chain Antibody]
The framework regions (FRs) of the VH chain of a single-chain antibody includes FR1, FR2, FR3, and FR4. As is well known, the amino acid sequences of the FRs of the VH chain also contribute to the binding capacity for an antigen.
The amino acid sequences of the FRs of the VH chain of the single-chain antibody in the present embodiment are not particularly limited, as long as an antibody constructed using the FR sequences binds to an antigen. The amino acid sequences of FR1, FR2, FR3, and FR4 are preferably the amino acid sequences of FR1, FR2, FR3, and FR4, respectively, of any one of the VH chains described in Examples in the present specification, in cases where the present method is carried out using a human serum-derived IgG polyclonal antibody or a human serum-derived IgA polyclonal antibody as the antigen, and a rabbit-derived single-chain antibody as the single-chain antibody. This is because an antibody constructed using such FR sequences has a high binding capacity for the antigen. Further, among these sequences, more preferred are amino acid sequences which allow an antibody constructed therewith to have a higher binding capacity for the antigen.
[Amino Acid Sequences Substantially Homologous to Amino Acid Sequences of FRs of VH Chain]
The description to be given here is the same as that given above in the section of “Amino Acid Sequences Substantially Homologous to Amino Acid Sequences of CDRs of VH Chain”.
[Framework Regions (FR) of VL Chain of Single-Chain Antibody]
The framework regions (FRs) of the VL chain of a single-chain antibody includes FR1, FR2, FR3, and FR4. As is well known, the amino acid sequences of the FRs of the VL chain also contribute to the binding capacity for an antigen.
The amino acid sequences of the FRs of the VL chain of the single-chain antibody in the present embodiment are not particularly limited, as long as an antibody constructed using the FR sequences binds to an antigen. The amino acid sequences of FR1, FR2, FR3, and FR4 are preferably the amino acid sequences of FR1, FR2, FR3, and FR4, respectively, of any one of the VL chains described in Examples in the present specification, in cases where the present method is carried out using a human serum-derived IgG polyclonal antibody or a human serum-derived IgA polyclonal antibody as the antigen, and a rabbit-derived single-chain antibody as the single-chain antibody. This is because an antibody constructed using such FR sequences has a high binding capacity for the antigen. Further, among these sequences, more preferred are amino acid sequences which allow an antibody constructed therewith to have a higher binding capacity for the antigen.
[Amino Acid Sequences Substantially Homologous to Amino Acid Sequences of FRs of VL Chain]
The description to be given here is the same as that given above in the section of “Amino Acid Sequences Substantially Homologous to Amino Acid Sequences of CDRs of VH Chain”.
The second embodiment in the first invention of the present invention is a method for producing an antibody, the method including the steps of:
performing screening by the screening method according the first embodiment;
determining the amino acid sequence of the screened single-chain antibody;
preparing a DNA sequence encoding the antibody based on the sequence of the variable region of the determined amino acid sequence;
expressing the prepared DNA sequence in a host cell.
<(1) Step of Performing Screening by Screening Method According to First Embodiment>
The present step is a step of performing screening by the screening method according the first embodiment. The description previously given for the first embodiment applies to the description of the present step.
<(2) Step of Determining Amino Acid Sequence of Screened Single-Chain Antibody>
The present step is a step of determining the amino acid sequence of the screened single-chain antibody. The method therefor is not limited, as long as the amino acid sequence of the screened single-chain antibody can be determined.
For example, the amino acid sequence can be determined based on the gene sequence determined by the previously described “gene sequencing step”.
<(3) Step of Preparing DNA Sequence Encoding Antibody Based on Sequence of Variable Region of Determined Amino Acid Sequence>
In the present step, the method for preparing a DNA sequence is not limited, as long as a DNA sequence encoding the antibody can be prepared, based on the sequence of the variable region of the determined amino acid sequence. Since codons encoding the respective amino acids are well known, the base sequence of DNA encoding a specific amino acid sequence can be easily identified.
There are a number of known methods for preparing a DNA sequence encoding the antibody. The DNA sequence can be prepared, for example, by ligating the DNA sequence encoding the variable region (V domain) of the amino acid sequence determined in the step of determining the amino acid sequence to DNA encoding a desired constant region (C domain), and the ligated DNA is incorporated into an expression vector. Alternatively, the DNA encoding the variable region (V domain) of the antibody can be incorporated into an expression vector containing DNA encoding the constant region. At this time, the DNA is incorporated into an expression vector, for example, so as to be expressed under the control of an expression regulatory region, such as an enhancer or promoter, and a host cell can be transformed with the thus prepared expression vector to produce the antibody.
The amino acid sequence of the constant region (C domain) to be used at this time may be derived from any animal, and there is no particular limitation on the animal. The amino acid sequence of the constant region (C domain) may be derived from an animal different from the animal from which the amino acid of the variable region (V domain) is derived. In cases where such a combination of amino acid sequences is used to produce an antibody, the resulting antibody is a chimeric antibody. Examples of the animal include humans, rats, mice, goats, sheep, cows, horses, dogs, cats, and monkeys. Among these, a human is preferred. In cases where the amino acid of the variable region (V domain) is derived from an animal other than a human, and the amino acid sequence of the constant region (C domain) is derived from a human, the resulting antibody produced by such a combination is a humanized antibody.
Further, an antibody to be encoded by the DNA sequence need not be an immunoglobulin, and may be, for example, an scFv, Fv, Fab, Fab′, or F(ab′)2.
(Encoding Humanized Antibody, DNA Sequence)
A description will be given below with reference to a DNA sequence encoding a humanized antibody. As described above, the animal from which the amino acid sequence of the constant region (C domain) is derived is not limited.
A humanized antibody is a modified antibody which is also referred to as a reshaped human antibody. In the present embodiment, a humanized antibody can be constructed by grafting the CDRs of the single-chain antibody screened by the screening method according to the first embodiment into the complementarity determining regions of a human antibody. Common genetic engineering techniques for producing such a humanized antibody are also known. For example, these methods can be found in WO 2013/125654, European Patent Application No. EP 239400, WO 96/02576, and the like.
In the present embodiment, a humanized antibody can be constructed, for example, as follows. Specifically, a DNA sequence designed to ligate the CDRs of the single-chain antibody screened by the screening method according to the first embodiment to the FRs of a human antibody is synthesized by PCR from several oligonucleotides prepared to have terminal overlapping regions. The resulting DNA sequence is ligated to the DNA sequence encoding the constant region of the human antibody. The ligated DNA is inserted into an expression vector, which is then incorporated into a host cell to allow the production of a humanized antibody.
The FRs of the human antibody to be ligated via the CDRs are selected in such a manner that the complementarity determining regions form an appropriate antigen-binding site. If necessary, amino acids in the framework regions of the variable region in the humanized antibody may be substituted so that the complementarity determining regions of the humanized antibody forms an appropriate antigen-binding site. The method therefor is disclosed, for example, in Sato K. et al., Cancer Research 1993, 53: 851-856, and the like. Further, the FRs may be replaced with framework regions derived from a human antibody of a different class or a subclass. The method therefor is disclosed, for example, in WO 99/51743.
When producing a humanized antibody, amino acids in the variable region (for example, FRs) and the constant region may be substituted with other amino acids. For example, the method described in The Journal of Japanese Society on Thrombosis and Hemostasis 4 (3): 193-200, 1993 may be used. As described in the above document, the determined amino acid sequence of the variable region may be compared with the amino acid sequences of the variable regions of human antibodies found in data banks to select a human antibody gene having a skeleton (FRs) with the highest similarity to that of the determined sequence, and then the higher order structure of the selected gene is analyzed using computer graphics, thereby determining the optimum amino acid sequence of the variable region. Further, it is also possible to carry out the substitution of amino acids, and the like, which are necessary for achieving an efficient antibody production, when inserting the DNA into an expression vector and then incorporating the vector into a host cell to produce an antibody.
The substitution of amino acids is, for example, a substitution of less than 15, less than 10, 8 or less, 7 or less, 6 or less, 5 or less, 4 or less, 3 or less, or 2 or less amino acids, preferably a substitution of 1 to 5 amino acids, and more preferably a substitution of 1 or 2 amino acids, and a substituted antibody should be functionally equivalent to an unsubstituted antibody. The substitution is preferably a conservative amino acid substitution, which is a substitution between amino acids having similar properties, such as those having similar electric charge, side chains, polarity, aromaticity, etc. Amino acids having similar properties can be classified, for example, into: basic amino acids (arginine, lysine, and histidine), acidic amino acids (aspartic acid and glutamic acid), uncharged polar amino acids (glycine, asparagine, glutamine, serine, threonine, cysteine, and tyrosine), non-polar amino acids (leucine, isoleucine, alanine, valine, proline, phenylalanine, tryptophan, and methionine), branched-chain amino acids (leucine, valine, and isoleucine), aromatic amino acids (phenylalanine, tyrosine, tryptophan, and histidine), and the like.
<(4) Step of Expressing Prepared DNA Sequence in Host Cell>
In the present step, the method for carrying out the step is not limited, as long as the DNA sequence prepared in the step of preparing a DNA sequence encoding the antibody can be expressed in a host cell.
For example, many of the host cells used for antibody production are derived from mammals, and those skilled in the art can select as appropriate a specific type of host cells which is most suitable for expressing a desired gene product. Examples of host cell lines which are commonly used include CHO-derived cell lines (Chinese hamster ovary cell lines), CV1 (monkey kidney cell line), COS (a derivative of CV1 doing SV40T antigen), SP2/0 (mouse myeloma cell line), P3x63-Ag3.653 (mouse myeloma cell line), 293 (human kidney cell line), and 293T (a derivative of 293 expressing SV40T antigen), but not particularly limited thereto. Host cell lines are available from various manufacturers, organizations such as ATCC, or organizations publishing papers cited in literature.
<(5) Optional Steps>
After the expression step in a host cell, a step of separating and purifying the resulting antibody may be carried out. The method therefor is not particularly limited, and any of known separation and purification methods may be combined as appropriate to carry out the separation and purification of the antibody.
Examples of the method include: methods utilizing a difference in electric charge, such as ion-exchange chromatography; methods primarily utilizing a difference in molecular weight, such as dialysis, ultrafiltration, gel filtration, and SDS-polyacrylamide gel electrophoresis; methods utilizing specific affinity, such as affinity chromatography; methods utilizing a difference in hydrophobicity, such as reverse-phase high performance liquid chromatography; methods utilizing a difference in isoelectric point such as isoelectric focusing; and the like.
<2. Second Invention>
The second invention of the present invention includes the following first to sixth embodiments.
The first embodiment: a single-chain antibody having a dissociation constant for a human serum-derived IgG polyclonal antibody of not more than 3.0×10−8 M.
The second embodiment: a separation agent for separating a human serum-derived IgG polyclonal antibody, the separation agent including: a carrier; and the single-chain antibody according to the first embodiment, which binds to the surface of the carrier via a chemical bond.
The third embodiment: a single-chain antibody having a dissociation rate constant for a human serum-derived IgA polyclonal antibody of not more than 1.0×10−3 s−1
The fourth embodiment: a separation agent for separating a human serum-derived IgA polyclonal antibody, the separation agent including: a carrier; and the single-chain antibody according to the third embodiment, which binds to the surface of the carrier via a chemical bond.
The fifth embodiment: a single-chain antibody having a dissociation rate constant for the L chain of a human-derived antibody of not more than 1.0×10−3 s−1
The sixth embodiment: a separation agent for separating a human-derived antibody, the separation agent including: a carrier; and the single-chain antibody according to the fifth embodiment, which binds to the surface of the carrier via a chemical bond.
The first embodiment in the second invention of the present invention is a single-chain antibody having a dissociation constant for a human serum-derived IgG polyclonal antibody of not more than 3.0×10−8 M.
The above described single-chain antibody is preferably also an antibody against a human serum-derived IgA polyclonal antibody, and more preferably has a dissociation rate constant for the human serum-derived IgA polyclonal antibody of not more than 1.0×10−3 s−1. Further, the single-chain antibody preferably binds to the L chain of such an antibody, and more preferably binds to the kappa chain of such an antibody.
The description previously given for the first invention applies to the description regarding other matters in the present embodiment.
The second embodiment in the second invention of the present invention is a separation agent for separating a human serum-derived IgG polyclonal antibody, the separation agent including: a carrier; and the single-chain antibody according to the first embodiment in the second invention, which binds to the surface of the carrier via a chemical bond.
[Separation Agent for Separating Human Serum-Derived IgG Polyclonal Antibody]
The single-chain antibody according to the first embodiment can be used as a separation agent for separating a human serum-derived IgG polyclonal antibody, utilizing the capacity of the single-chain antibody to bind to the antibody. The above described separation agent can be used for the purification or removal of the antibody, as well as for the diagnosis, treatment, examination and the like utilizing the antibody.
The separation agent according to the present embodiment has a form in which the single-chain antibody according to the first embodiment is immobilized on a solid phase support which is insoluble in water.
[Water-Insoluble Carrier]
Examples of the water-insoluble carrier to be used include: inorganic carriers such as glass beads and silica gels; organic carriers composed of synthetic polymers such as crosslinked polyvinyl alcohols, crosslinked polyacrylates, crosslinked polyacrylamides and crosslinked polystyrenes, and/or polysaccharides such as crystalline cellulose, crosslinked cellulose, crosslinked agarose and crosslinked dextran; as well as composite carriers obtained by combining these carriers, such as organic-organic and organic-inorganic composite carriers. Among these, a hydrophilic carrier is preferred because it has a relatively low non-specific adsorption, and a good selectivity for the single-chain antibody according to the first embodiment. The hydrophilic carrier as used herein refers to a carrier which has a contact angle with water, as measured when the compound(s) constituting the carrier is/are formed into a plate-like shape, of 60 degrees or lower. Representative examples of such a carrier include carriers composed of: polysaccharides such as cellulose, chitosan and dextran; polyvinyl alcohol; a saponified product of ethylene-vinyl acetate copolymer; polyacrylamide; polyacrylic acid; polymethacrylic acid; polymethylmethacrylate; polyacrylic acid-grafted polyethylene; polyacrylamide-grafted polyethylene; and glass.
Examples of commercially available products thereof include: GCL2000 and GC700, which are porous cellulose gels; Sephacryl S-1000, obtained by covalently crosslinking allyl dextran and methylene bisacrylamide; Toyopearl, which is an acrylate-based carrier; Sepharose CL4B, which is an agarose-based crosslinked carrier; Eupergit C250L, which is a polymethacrylamide activated with epoxy groups; and the like. Note, however, that the carrier to be used in the present embodiment is not limited only to these carriers and activated carriers. Each of the above described carriers may be used alone, or arbitrarily selected two or more kinds of these carriers may be mixed for use. Further, the water-insoluble carrier to be used in the present embodiment preferably has a large surface area, in terms of the purposes and methods of using the present separation agent. In other words, the carrier to be used is preferably a porous carrier which has a number of pores of an appropriate size.
The form of the carrier can be selected arbitrarily, and any of the carriers in the form of beads, fibers, membranes (including hollow fibers) and the like can be used. Among these, a carrier in the form of beads is particularly preferably used, because one having a specific exclusion limit molecular weight can be easily formed. A carrier in the form of beads having an average particle size of from 10 to 2,500 μm is easy to use. In particular, preferred is a carrier in the form of beads having an average particle size within the range of from 25 μm to 800 μm, because the immobilization reaction of the single-chain antibody on such a carrier can be easily performed.
In addition, if a functional group which can be used for the immobilization reaction of the single-chain antibody are present on the carrier surface, it is convenient for the immobilization of the single-chain antibody. Representative examples of the functional group include hydroxyl group, amino group, aldehyde group, carboxyl group, thiol group, silanol group, amide group, epoxy group, succinylimide group, acid anhydride groups, iodoacetyl group, and the like.
When the single-chain antibody is immobilized on the carrier as described above, it is preferred that the steric hindrance of the single-chain antibody be reduced so as to improve the separation efficiency. In addition, it is more preferred that the single-chain antibody be immobilized on the carrier via a hydrophilic spacer, so as to reduce non-specific binding. As the hydrophilic spacer, it is preferable to use, for example, a polyalkylene oxide derivative substituted at both ends with a carboxyl group, an amino group, an aldehyde group, an epoxy group, etc.
The method and conditions for immobilizing the single-chain antibody to be incorporated into the carrier and an organic compound to be used as a spacer, are not particularly limited. Methods commonly used for immobilizing a protein or a peptide on a carrier will be exemplified below. For example, the immobilization may be carried out by a method in which a carrier is allowed to react with cyanic bromide, epichlorohydrin, diglycidyl ether, tosyl chloride, tresyl chloride, hydrazine or the like to activate the carrier (namely, functional groups originally present on the carrier are replaced with functional groups which more easily react with the single-chain antibody), thereby allowing the carrier to react with the single-chain antibody and the single-chain antibody to be immobilized on the carrier. Alternatively, a method may be used in which a condensation reagent such as carbodiimide, or a reagent containing a plurality of functional groups within the molecule, such as glutaraldehyde, is added to a system in which a carrier and the single-chain antibody are present, followed by condensation and crosslinking, thereby immobilizing the single-chain antibody on the carrier. However, it is more preferable to use a method which allows the single-chain antibody to be immobilized on a carrier such that the single-chain antibody is not easily desorbed from the carrier during the sterilization or use of the separation agent.
Specific examples of the separation agent for separating a human serum-derived IgG polyclonal antibody and the method for producing the same include HiTrap NHS-activated HP Columns (manufactured by GE Healthcare Inc.), and the method for immobilizing the single-chain antibody according to the first embodiment, using the same, as will be described in Example 8. Stated simply, the carboxyl group of the Sepharose (an agarose carrier in the form of beads) in the column is esterified with NHS, and allowed to form an amide bond with an amino group of the single-chain antibody according to the first embodiment which has been purified, thereby immobilizing the single-chain antibody. Unreacted NHS esters can be blocked by addition of ethanolamine.
[Other Matters]
The descriptions previously given for the first invention and the first embodiment in the second invention apply to the description regarding other matters in the present embodiment.
The third embodiment in the second invention of the present invention is a single-chain antibody having a dissociation rate constant for a human serum-derived IgA polyclonal antibody of not more than 1.0×10−3 s−1.
The above described single-chain antibody is preferably also an antibody against a human serum-derived IgG polyclonal antibody, and more preferably has a dissociation constant for the human serum-derived IgG polyclonal antibody of not more than 3.0×10−8 M. Further, the single-chain antibody preferably binds to the L chain of such an antibody, and more preferably binds to the kappa chain of such an antibody.
The description previously given for the first invention applies to the description regarding other matters in the present embodiment.
The fourth embodiment in the second invention of the present invention is a separation agent for separating a human serum-derived IgA polyclonal antibody, the separation agent including: a carrier; and the single-chain antibody according to the third embodiment in the second invention, which binds to the surface of the carrier via a chemical bond.
The descriptions previously given for the first invention, the second embodiment in the second invention, and the third embodiment in the second invention apply to the description regarding other matters in the present embodiment.
The fifth embodiment in the second invention of the present invention is a single-chain antibody having a dissociation rate constant for the L chain of a human-derived antibody of not more than 1.0×10−3 s−1
The above described single-chain antibody is preferably an antibody against a human serum-derived IgG polyclonal antibody and/or a human serum-derived IgA polyclonal antibody, and more preferably has a dissociation constant for the human serum-derived IgG polyclonal antibody of not more than 3.0×10−8 M, and/or a dissociation rate constant for the human serum-derived IgA polyclonal antibody of not more than 1.0×10−3 s−1. Further, the single-chain antibody preferably binds to the kappa chain of such an antibody.
The description previously given for the first invention applies to the description regarding other matters in the present embodiment.
The sixth embodiment in the second invention of the present invention is a separation agent for separating a human-derived antibody, the separation agent including: a carrier; and the single-chain antibody according to the fifth embodiment in the second invention, which binds to the surface of the carrier via a chemical bond.
The descriptions previously given for the first invention, the second embodiment in the second invention, and the fifth embodiment in the second invention apply to the description regarding other matters in the present embodiment.
The present invention will now be described more specifically by way of Examples. However, the present invention is in no way limited by the following Examples, as long as the gist of the present invention is not deviated. Note that there are cases where Examples and Comparative Examples are not described in their numerical order, for convenience sake.
<1. Model Study>
Before describing Examples of the screening method according to the first invention of the present invention, a description will be given below regarding the method for screening a mouse-derived single-chain antibody which binds to a human serum-derived IgG polyclonal antibody (hereinafter, sometimes referred to as an “anti-human serum-derived IgG polyclonal antibody-mouse-derived single-chain antibody”), from a phage library. A description will also be given regarding the case in which a library of phages not presenting the mouse-derived single-chain antibody is used, as a comparative study. Further, for each of the above cases, a study in which multilamellar liposomes were used and a study in which an immunotube was used will be described.
<1-1. Coupling of Human Serum-Derived IgG Polyclonal Antibody to Multilamellar Liposomes>
A quantity of 10 μmol of dipalmitoylphosphatidylcholine (DPPC), 1 μmol of dicetyl phosphate (DCP), 0.5 μmol of N-(4-(p-maleimidophenyl)butyryl)dipalmitoylphosphatidylethanolamine (MPB-DPPE) were dissolved in 5 ml of chloroform. Then the chloroform in the resulting solution was removed by distillation in a 100 ml eggplant flask, under reduced pressure.
Subsequently, the resulting thin film of phospholipid formed on the inner wall of the flask was hydrated with 3 ml of PBS at 50° C., to form multilamellar liposomes (MLVs). The resultant was centrifuged at 20,000 g and at 25° C. for two minutes, and the supernatant was removed. This operation was repeated two more times.
The resulting multilamellar liposomes were suspended in 3 ml of PBS and stored at 4° C. (the resultant is sometimes referred to as “reactive MLVs”). A quantity of 1 ml of reactive MLVs was centrifuged at 20,000 g and at 25° C. for two minutes. A human serum-derived IgG polyclonal antibody (#I4506; manufactured by Sigma-Aldrich Co. LLC.) was dissolved in PBS to a concentration of 1 mg/ml, and to the resulting solution, the pellets of the reactive MLVs obtained after the centrifugation were dispersed.
To the resultant, 2-iminothiolane hydrochloride (manufactured by Sigma-Aldrich Co. LLC.) was added, in an amount 10 times the amount of the human serum-derived IgG polyclonal antibody, in molar ratio, followed by incubation at 25° C. for three hours or more, while stirring. Thereafter, centrifugation was carried out at 20,000 g and at 25° C. for two minutes, the supernatant was removed, and the resultant was suspended in 1 ml of PBS. An operational process consisting of the above described centrifugation, removal of supernatant, and suspension in 1 ml of PBS, as one unit, was repeated three more times.
The resulting suspension was stored at 4° C., to be used as human serum-derived IgG polyclonal antibody-immobilized MLVs. The amount of the human serum-derived IgG polyclonal antibody immobilized on the MLVs was quantified using DC Protein Assay.
<1-2. Immobilization of Human Serum-Derived IgG Polyclonal Antibody on Tube>
A quantity of 1 ml of a solution of a human serum-derived IgG polyclonal antibody (#I4506; manufactured by Sigma-Aldrich Co. LLC.), prepared with PBS to a concentration of 10 μg/ml, was added to an immunotube (Maxisorp (registered trademark); manufactured by Nunc), followed by incubation at 4° C. overnight. Subsequently, the tube was washed with PBS five times, and 1 ml of 2% BSA-PBS was added thereto, followed by incubation for one hour.
Before mixing with a phage library, the tube was washed with PBS five more times, and then a phage library solution was added thereto and mixed for use.
It has been shown in Non-patent Document 1 that, although it is the result obtained in the case of using a rabbit-serum derived IgG polyclonal antibody, the ratio of the antibody non-specifically bound to a tube when the antibody is immobilized on the tube, is markedly higher as compared to the ratio of the antibody non-specifically bound to multilamellar liposomes when the antibody is immobilized on the multilamellar liposomes. Those skilled in the art can easily understand that the same applies to the case in which a human serum-derived IgG polyclonal antibody is used.
<1-3. Preparation of Library of Phages Presenting Anti-Human Serum-Derived IgG Polyclonal Antibody-Mouse-Derived Single-Chain Antibody>
A DNA containing a gene sequence of pelB leader, an Nco I site, an Spe I site, a gene sequence of flexible linker (G4S)3, a BamH I site, a Not I site, a gene sequence of FLAG-tag, a gene sequence of c-myc-tag, an Amber stop codon (TAG), and a gene sequence of gIIIp coat protein (250 amino acid residues on the N-terminus are deleted) was synthesized by a commissioned service, and the DNA was inserted into the Xba I/BamH I sites of pT7 Blue (manufactured by Merck KGaA). The thus obtained pT7 Blue recombinant phagemid vector was named as pPLFMAΔ250gIIIp, and used in a series of studies using the phage display method.
The gene of the anti-human serum-derived IgG polyclonal antibody-mouse-derived single-chain antibody determined by a mouse hybridoma CRL-1786 cell line (ATCC) was amplified by PCR, and inserted into the Nco I/Not I sites of the recombinant phagemid vector pPLFMAA250gIIIp.
The recombinant phagemid vector was used to transform Escherichia coli TG1 cells, and the transformed cells were inoculated in 10 ml of 2×YT medium (containing 1% glucose and 50 mg/L ampicillin). The cells were cultured overnight in a 200 ml Erlenmeyer flask, at 200 rpm and at 37° C. (preculture).
The precultured liquid was inoculated in 50 ml of 2×YT medium (containing 1% glucose and 50 mg/L ampicillin) so as to achieve an OD 600 of 0.1, followed by culturing at 30° C. with shaking at 200 rpm. After culturing the cells until the OD reached around 1.0, a helper phage, VCSM13 was added to the culture liquid so as to achieve a multiplicity of infection (MOI) of 20, followed by incubation at 37° C. for 30 minutes. Following centrifugation at 3,000 g and at 37° C. for 10 minutes, the supernatant was removed, and the resulting cells were gently suspended in 50 ml of 2×YT medium (containing 50 mg/L ampicillin and 35 mg/L kanamycin). The resulting suspension was shaken at 200 rpm and at 30° C. for 12 hours or more, thereby allowing phages presenting the anti-human serum-derived IgG polyclonal antibody-mouse-derived single-chain antibody to be produced in the culture supernatant.
The supernatant was collected by centrifugation, concentrated by PEG precipitation, and resuspended in 1 ml of PBS, to obtain a library of phages presenting the anti-human serum-derived IgG polyclonal antibody-mouse-derived single-chain antibody.
<1-4. Preparation of Library of Non-Presenting Phages>
The same procedure as in the above described section 1-3 was carried out, except that the recombinant phagemid vector pPLFMAA250gIIIp into which the gene of the anti-human serum-derived IgG polyclonal antibody-mouse-derived single-chain antibody was not inserted, was used to transform Escherichia coli TG1 cells, thereby obtaining non-presenting phages, namely, phages not presenting the anti-human serum-derived IgG polyclonal antibody-mouse-derived single-chain antibody.
<1-5. Panning>
(Preparation of Pseudo-Phage Library)
The library of phages presenting the anti-human serum-derived IgG polyclonal antibody-mouse-derived single-chain antibody, and the library of non-presenting phages, obtained in the above described sections 1-3 and 1-4, respectively, were mixed at the ratios shown in Table 1, to prepare pseudo-phage libraries.
TABLE 1
Composition of the pseudo-phage library
cfu/ml
Condition
cfu/ml
ratio
Condition 1
Library of phages presenting
8.8 × 108
1
anti-human serum-derived IgG
polyclonal antibody-mouse-
derived single-chain antibody
Non-presenting phages
4.7 × 1014
540,000
Condition 2
Library of phages presenting
8.8 × 107
1
anti-human serum-derived IgG
polyclonal antibody-mouse-
derived single-chain antibody
Non-presenting phages
4.7 × 1014
5,400,000
(Panning Using Human Serum-Derived IgG Polyclonal Antibody-Immobilized MLVs)
Panning was carried out as follows, using the pseudo-phage library prepared according to Condition 1, and using the human serum-derived IgG polyclonal antibody-immobilized MLVs prepared in the above section 1-1.
(Rounds)
First, operations to be carried out in each of the rounds will be described.
The human serum-derived IgG polyclonal antibody-immobilized MLVs were added in an amount to achieve an IgG content of 10 μg, followed by vortexing. Following centrifugation at 20,000 g and at 25° C. for two minutes, the supernatant was removed, and then 0.9 ml of 2% BSA-PBS was added to the resultant for resuspension.
Meanwhile, a solution of the pseudo-phage library was centrifuged at 20,000 g and at 25° C. for two minutes, and the supernatant was collected. A quantity of 100 μl of the supernatant was added to a tube, followed by vortexing. The resultant was then inversion mixed at 25° C. for one hour using a rotator, to allow a binding reaction between the human serum-derived IgG polyclonal antibody-immobilized MLVs and the pseudo-phage library to proceed.
The binding reaction liquid obtained above and 1 ml of 2% BSA-PBS were mixed, and the mixture was centrifuged at 20,000 g and at 25° C. for two minutes to remove the supernatant (washing). The washing operation was repeated five times.
(Recovery of Phages Selected by Panning)
To the human serum-derived IgG polyclonal antibody-immobilized MLVs in the above described tube, 0.9 ml of 10 mM glycine-HCl (pH 1.5) was added for suspension, and the resulting suspension was transferred to a BSA-blocked tube. Subsequently, the tube was further inversion mixed at room temperature (or at 4° C.) for 10 minutes, thereby eluting the phages.
A quantity of 0.9 ml of the phage eluent collected from the above tube and 0.1 ml of a 2M Tris-HCl solution were mixed to neutralize the phage eluent.
Meanwhile, a culture liquid of Escherichia coli TG1 cells were inoculated in 10 ml of fresh LB medium so as to achieve an OD of 0.1, followed by culturing at 30° C.
A quantity of 1 ml of the neutralized eluent and 1 ml of the culture liquid of Escherichia coli TG1 cells which had been cultured were mixed, followed by incubation at 37° C. for one hour. After the incubation, the cells was added to 2×YT medium (containing 1% glucose and 50 mg/L ampicillin), and cultured at 30° C. and at 200 rpm, until the OD 600 reached 1.0.
To the resulting culture liquid, a helper phage VCSM13 was added to achieve a multiplicity of infection (MOI) of 20, followed by incubation at 37° C. for 30 minutes. After centrifuging the culture liquid at 1,500 rpm and at 30° C. for 15 minutes, the supernatant was discarded, and the cells were redispersed in 50 ml of 2×YT medium (containing 50 mg/L ampicillin and 50 mg/L kanamycin). The cells were then cultured at 30° C. and at 200 rpm for 12 hours, to allow phages to be produced in the culture supernatant.
Following subsequent centrifugation at 1,500 rpm and at 30° C. for 15 minutes, the supernatant was collected, and then concentrated and purified by PEG precipitation. Finally, the resultant was dispersed in 1 ml of PBS, followed by centrifugation to remove aggregates.
A series of operations up to this point are defined as one round. When the above described operations were carried out, it is regarded that Round 1 has been completed.
Thereafter, the above described round was repeated three more times. In other words, the procedure up to Round 4 was carried out. From the colonies obtained in each of the rounds, phagemid DNAs were recovered.
The same procedure as in Example 1-1 was carried out as Example 1-2, except that the pseudo-phage library prepared according to Condition 2 was used.
Panning was carried out as follows, using the pseudo-phage library prepared according to Condition 1, and using the human serum-derived IgG polyclonal antibody-immobilized tube prepared in the above section 1-2, instead of the human serum-derived IgG polyclonal antibody-immobilized MLVs.
(Rounds)
Operations to be carried out in each of the rounds will be described.
As described in the above 1-2, 1 ml of a solution of a human serum-derived IgG polyclonal antibody (#I4506; manufactured by Sigma-Aldrich Co. LLC.), prepared with PBS to a concentration of 10 μg/ml, was added to an immunotube (Maxisorp (registered trademark); manufactured by Nunc), followed by incubation at 4° C. overnight. Subsequently, the tube was washed with PBS five times, and 1 ml of 2% BSA-PBS was added thereto, followed by incubation for one hour.
Thereafter, the tube was washed with PBST five times, and 900 μl of 2% BSA-PBST, and then 100 μl of a solution of the pseudo-phage library were added thereto, followed by incubation at 25° C. for one hour.
(Recovery of Phages Selected by Panning)
A culture liquid of Escherichia coli TG1 cells were inoculated in 10 ml of fresh LB medium so as to achieve an OD of 0.1, followed by culturing at 30° C.
A quantity of 1 ml of the eluent and 1 ml of the culture liquid of Escherichia coli TG1 cells which had been cultured were mixed, followed by incubation at 37° C. for one hour. After the incubation, the cells was added to 2×YT medium (containing 1% glucose and 50 mg/L ampicillin), and cultured at 30° C. and at 200 rpm, until the OD 600 reached 1.0.
To the resulting culture liquid, a helper phage VCSM13 was added to achieve a multiplicity of infection (MOI) of 20, followed by incubation at 37° C. for 30 minutes. After centrifuging the culture liquid at 1,500 rpm and at 30° C. for 15 minutes, the supernatant was discarded, and the cells were redispersed in 50 ml of 2×YT medium (containing 50 mg/L ampicillin and 50 mg/L kanamycin). The cells were then cultured at 30° C. and at 200 rpm for 12 hours, to allow phages to be produced in the culture supernatant.
Following subsequent centrifugation at 1,500 rpm and at 30° C. for 15 minutes, the supernatant was collected, and then concentrated and purified by PEG precipitation. Finally, the resultant was dispersed in 1 ml of PBS, followed by centrifugation to remove aggregates.
A series of operations up to this point are defined as one round. When the above described operations were carried out, it is regarded that Round 1 has been completed.
Thereafter, the above described round was repeated three more times. In other words, the procedure up to Round 4 was carried out. From the colonies obtained in each of the rounds, phagemid DNAs were recovered.
The same procedure as in Comparative Example 1-1 was carried out as Comparative Example 1-2, except that the pseudo-phage library prepared according to Condition 2 was used.
<1-6. Confirmation of Presence or Absence of Gene of Anti-Human Serum-Derived IgG Polyclonal Antibody-Mouse-Derived Single-Chain Antibody>
The presence or absence of the gene of the anti-human serum-derived IgG polyclonal antibody-mouse-derived single-chain antibody was confirmed in the phagemid DNAs recovered in Example 1-1, Example 1-2, Comparative Example 1-1, and Comparative Example 1-2.
The obtained phagemid DNAs were separated by electrophoresis using 1% agarose gel, and visualized by ethidium bromide staining. The migration distances of the phagemid DNAs were compared against the migration distance of the DNA of the phagemid vector (pPLFMAA250gIIIp) into which the gene of the anti-human serum-derived IgG polyclonal antibody-mouse-derived single-chain antibody was not inserted, and the presence or absence of the gene of the anti-human serum-derived IgG polyclonal antibody-mouse-derived single-chain antibody was visually confirmed.
<1-7. Panning Results>
Table 2-1 and Table 2-2 show the number of phages before and after the panning, and the recovery rate of the phages, which is the rate of the number of the phages after the panning to the number of the phages before the panning, in each of the rounds 1 to 4.
Further, Table 3 shows the ratio of the number of positive clones (namely, the number of clones containing the gene of the anti-human serum-derived IgG polyclonal antibody-mouse-derived single-chain antibody), with respect to the total number of clones obtained, in each of the rounds 1 to 4. The above described ratio is shown in
TABLE 2-1
Round 1
Round 2
Before
After
Recovery
Before
After
Recovery
Panning
Panning
Rate
Panning
Panning
Rate
(cfu/ml)
(cfu/ml)
(%)
(cfu/ml)
(cfu/ml)
(%)
Condition 1
Example 1-1
4.7E+14
2.8E+04
6.0E−09
4.2E+12
1.1E+06
2.6E−05
Comparative
4.7E+14
8.1E+05
1.7E−07
1.9E+12
1.4E+06
7.4E−05
Example 1-1
Condition 2
Example 1-2
4.7E+14
7.4E+04
1.6E−08
3.1E+13
1.5E+05
4.8E−07
Comparative
4.7E+14
1.3E+05
2.8E−08
4.0E+12
6.0E+06
1.5E−04
Example 1-2
TABLE 2-2
Round 3
Round 4
Before
After
Recovery
Before
After
Recovery
Panning
Panning
Rate
Panning
Panning
Rate
(cfu/ml)
(cfu/ml)
(%)
(cfu/ml)
(cfu/ml)
(%)
Condition 1
Example 1-1
2.8E+12
1.3E+07
4.6E−04
1.2E+14
2.4E+06
2.0E−06
Comparative
5.2E+12
2.0E+06
3.8E−05
2.0E+12
9.8E+06
4.9E−04
Example 1-1
Condition 2
Example 1-2
6.4E+12
5.9E+05
9.2E−06
1.0E+14
8.4E+06
8.3E−06
Comparative
3.2E+12
1.2E+06
3.8E−05
7.3E+12
2.1E+06
2.9E−05
Example 1-2
TABLE 3
Round 1
Round 2
Round 3
Round 4
Number
Number
Number
Number
of positive
Ratio
of positive
Ratio
of positive
Ratio
of positive
Ratio
clones
(%)
clones
(%)
clones
(%)
clones
(%)
Condition 1
Example 1-1
0
0
1
17
6
100
6
100
Comparative
0
0
0
0
0
0
0
0
Example 1-1
Condition 2
Example 1-2
0
0
0
0
3
50
6
100
Comparative
0
0
0
0
0
0
0
0
Example 1-2
The above results revealed that the use of the method in which the human serum-derived IgG polyclonal antibody as an antigen was coupled to multilamellar liposomes enables a more efficient panning, as compared to using the method in which the human serum-derived IgG polyclonal antibody was immobilized on a tube.
<2. Method for Screening Rabbit-Derived Single-Chain Antibody which Binds to Human Serum-Derived IgG Polyclonal Antibody>
A description will be given below regarding the method for screening a rabbit-derived single-chain antibody which binds to a human serum-derived IgG polyclonal antibody (hereinafter, sometimes referred to as an “anti-human serum-derived IgG polyclonal antibody-rabbit-derived single-chain antibody”), from a phage library.
<1-2. Coupling of Human Serum-Derived IgG Polyclonal Antibody to Multilamellar Liposomes>
Human serum-derived IgG polyclonal antibody-immobilized MLVs were prepared in the same manner as described in the above section 1-1.
<2-2. Preparation of Library of Phages Presenting Anti-Human Serum-Derived IgG Polyclonal Antibody-Rabbit-Derived Single-Chain Antibodies>
First, a European rabbit was immunized with a human serum-derived IgG polyclonal antibody (#I4506; manufactured by Sigma-Aldrich Co. LLC.) by a known method. The total RNA was extracted from the spleen of the immunized rabbit.
Using Superscript (registered trademark) IV Reverse Transcriptase (manufactured by Thermo Fisher Scientific) as a reverse transcriptase, cDNA was prepared from the total RNA. Using the cDNA as a template, and the sequences of SEQ ID NOs: 1 to 11 as primers, the genes of the variable regions (VH domains) of the heavy chains (H chains), and genes of the variable regions (VL domains) of the light chains (L chains) were amplified.
The thus amplified VL genes were introduced into the BamH I/Not I sites of pPLFMAΔgIIIp vectors, to be used as VL library vectors. Escherichia coli TG1 cells were used as the host cells.
Next, the VL library vectors were purified from the Escherichia coli cells, and the amplified VH genes were introduced into the Nco I/Spe I sites, to obtain phage library vectors (2.0×107 colonies) presenting anti-human serum-derived IgG polyclonal antibody-rabbit-derived single-chain antibodies. The host cells used at this time were also Escherichia coli TG1 cells.
Subsequently, the Escherichia coli TG1 cells containing the phage library vectors were inoculated in 50 ml of 2×YT medium (containing 1% glucose and 50 mg/L ampicillin), and then cultured at 30° C. with shaking at 200 rpm, until the OD reached 1. To the resulting culture liquid, a helper phage VCSM13 was added to achieve a multiplicity of infection: MOI of 20, followed by incubation at 37° C. for one hour. Following centrifugation at 1,500 rpm and at 30° C. for 15 minutes, the supernatant was discarded, and the cells were suspended in 50 ml of 2×YT medium (containing 50 mg/L ampicillin and 50 mg/L kanamycin), and cultured at 30° C. and at 200 rpm for 12 hours or more, to allow phages to be produced in the culture supernatant.
The resultant was centrifuged twice at 10,000 g and at 4° C. for 15 minutes, and the supernatant was collected as a phage library. Subsequently, the phage library is concentrated by PEG precipitation, and then dispersed in 1 ml of 1×PBS.
<2-3. Panning>
Panning was carried out as follows, using the phage library prepared in the above section 2-2, and the human serum-derived IgG polyclonal antibody-immobilized MLVs prepared in the above section 2-1.
(Rounds)
Operations to be carried out in each of the rounds will be described.
To a 1.5 ml eppendorf tube, 1 ml of 2% BSA-PBS was added, and blocking was carried out at room temperature for one hour or more. The above described blocking was performed for all the tubes to be used. The human serum-derived IgG polyclonal antibody-immobilized MLVs were added in an amount to achieve an IgG content of 10 μg, followed by vortexing. Following centrifugation at 20,000 g and at 4° C. for two minutes, the supernatant was removed. The phage library diluted 10-fold with 1 ml of 2% BSA-PBS was added to the resultant, and the mixture was incubated overnight at 4° C. under inversion rotation.
Subsequently, the resultant was centrifuged at 20,000 g at 4° C. for two minutes, and the supernatant was removed. A quantity of 1 ml of 2% BSA-PBS was added to the resultant for suspension, and the mixture was transferred to another eppendorf tube. An operational process consisting of the above described centrifugation, removal of supernatant, suspension with 2% BSA-PBS, and transfer to another eppendorf tube, as one unit, was repeated three times in total.
(Recovery of Phages Selected by Panning)
Subsequently, the tube was centrifuged at 20,000 g and at 4° C. for two minutes, and the supernatant was removed. A quantity of 0.9 ml of 10 mM glycine-HCl (pH 1.5) was added to the tube for suspension, and the resulting solution was transferred to another eppendorf tube. The tube was incubated at 4° C. for 10 minutes under inversion rotation, thereby eluting the phages.
The resultant was centrifuged at 20,000 g and at 4° C. for two minutes, and the supernatant was transferred to another eppendorf tube. Further, 0.1 ml of 2M Tris-HCl (pH 8.0) was added to the resultant, thereby neutralizing the phage eluent.
To the neutralized phage eluent, 1 ml of the culture liquid of Escherichia coli TG1 cells which had been cultured in advance, which cells were in the middle stage of the exponential growth, were added, followed by incubation at 37° C. for 30 minutes.
The resulting solution was suspended in 2×YT medium (containing 1% glucose and 50 mg/L ampicillin), followed by culturing at 30° C. with shaking at 200 rpm. After growing the cells until the OD reached around 1.0, VCSM13 was added to the cells so as to achieve a multiplicity of infection (MOI) of 20, and the mixture was incubated at 37° C. for 30 minutes, followed by centrifugation at 3,000 g and at 30° C. for 10 minutes.
Following centrifugation at 1,500 rpm and at 30° C. for 15 minutes, the supernatant was removed, and the E. coli cells were suspended in 50 ml of 2×YT medium (containing 50 mg/L ampicillin and 50 mg/L kanamycin). Thereafter, the cells were cultured at 200 rpm and at 30° C. for 12 hours, to allow phages to be produced in the culture supernatant.
Subsequently, the resultant was centrifuged at 20,000 g at 4° C. for two minutes, the supernatant was collected, and PEG precipitation was carried out (twice), followed by dispersion in 1 ml of PBS. Finally, the resulting dispersion was centrifuged at 20,000 g and at 4° C. for two minutes, and the supernatant was collected as a phage solution.
A series of operations up to this point are defined as one round. When the above described operations were carried out, it is regarded that Round 1 has been completed.
Thereafter, the above described round was repeated two more times. In other words, the procedure up to Round 3 was carried out. From the colonies obtained in each of the rounds, phagemid DNAs were recovered.
The same procedure as in Example 2 was carried out as Comparative Example 2, except that multilamellar liposomes which had not been coupled with the human serum-derived IgG polyclonal antibody were used.
<2-4. Recovery of Phages to Gene Sequencing>
The presence or absence of the genes of the anti-human serum-derived IgG polyclonal antibody-rabbit-derived single-chain antibodies was confirmed in the phagemid DNAs recovered in Example 2 and Comparative Example 2.
The obtained phagemid DNAs were separated by electrophoresis using 1% agarose gel, and visualized by ethidium bromide staining. The migration distances of the phagemid DNAs were compared against the migration distance of the DNA of the phagemid vector (pPLFMAA250gIIIp) into which none of the genes of the anti-human serum-derived IgG polyclonal antibody-rabbit-derived single-chain antibodies was inserted, and the presence or absence of the genes of the anti-human serum-derived IgG polyclonal antibody-rabbit-derived single-chain antibodies was visually confirmed. The sequencing of the phagemid vectors in which the insertion of the genes was confirmed was carried out by DNA sequence analysis (by a commissioned service).
The determination of the CDRs in the above genes was carried out using Vquest search engine available at IMGT (http://www.imgt.org/).
<2-5. Panning Results>
The above results revealed that, in Example 2, a marked increase in the recovery rate was already observed at the completion of Round 2. It is to be noted that, in the method using a common immunotube, such a high recovery rate (%) cannot be obtained at least until the completion of Round 3 to Round 4. In other words, it has been found out that the use of multilamellar liposomes allows for a markedly efficient panning as compared to using a conventional technique.
<3-1. Evaluation of Antigen-Binding Activity 1>
For the rabbit-derived single-chain antibodies obtained from the pellet portion of the phagemid-containing Escherichia coli cells (namely, the entire phages contained in the Escherichia coli cells which did not form single colonies and contained in the pellets) collected in each of the rounds, the evaluation of the antigen-binding activity was carried out as follows.
To Maxisorp (registered trademark) (manufactured by Thermo Fisher Scientific) plates, 100 μl of PBS was added, such that a human IgG1 (#I5154; manufactured by Sigma-Aldrich Co. LLC.), a human IgG2 (#I5404; manufactured by Sigma-Aldrich Co. LLC.), a human IgG3 (#I5654; manufactured by Sigma-Aldrich Co. LLC.), a human IgG4 (#I4639; manufactured by Sigma-Aldrich Co. LLC.), and a human IgA (#I4036; manufactured by Sigma-Aldrich Co. LLC.), each achieved a final concentration of 5 μg/ml, and the plates were incubated overnight at 4° C. (immobilization of antigen).
Subsequently, the antigen-immobilized plates were washed with PBS, and 300 μl of 10% Blocking One-PBS (manufactured by Nakalai Tesque, Inc.) was added to the plates. The plates were then incubated at 25° C. for one hour (blocking), and washed with PBST.
Meanwhile, to 25 ml of each of the phagemid-containing Escherichia coli pellets obtained before the panning, at the completion of Round 1, at the completion of Round 2, and at the completion of Round 3 in Example 2, 2.5 ml of Bugbuster (registered trademark) (manufactured by Merck KGaA) and 2.5 μL Benzonase Nuclease (registered trademark) (manufactured by Merck KGaA) were added to lyse the cells. Then, the resultants were centrifuged at 10,000 g and at 4° C. for 15 minutes, and the supernatants were collected.
The supernatants were each diluted 10-fold with 10% Blocking One-PBST, and 100 μl each of the diluted supernatants were added to the above described plates which had been blocked and washed with PBST, followed by incubation at 25° C. for one hour.
Subsequently, the plates were washed with PBST, and 100 μl of an HRP-labeled anti-c-myc antibody diluted 10,000-fold with 10% Blocking One-PBST was added to each of the plates, followed by incubation at 25° C. for one hour.
The plates were then washed with PBST, and 100 μl of a TMB solution was added to each plate, followed by incubation for five minutes. Thereafter, 100 μl of 0.3 M sulfuric acid was added to each plate to terminate the reaction.
The absorbance at 450 nm was measured using a microplate reader. At this time, a wavelength of 650 nm was used as the secondary wavelength.
The results are shown in
Further, it has been confirmed that the phages which also bind specifically to the human IgA antibody, in addition to the human IgG1 antibody, the human IgG2 antibody, the human IgG3 antibody, and the human IgG4 antibody, are concentrated at the completion of Round 2.
<3-2. Evaluation of Antigen-Binding Activity 2>
The evaluation of the antigen-binding activity was carried out for the rabbit-derived single-chain antibodies obtained from the colonies of the phagemid-containing Escherichia coli cells collected in each of the rounds, as follows.
Each of the colonies of the phagemid-containing Escherichia coli cells collected before the panning, at the completion of Round 1, at the completion of Round 2, and at the completion of Round 3 in Example 2 was inoculated in a well of a 96-well deep well plate, in 1 ml of Overnight Express (registered trademark; manufactured by Merck KGaA) medium, and cultured at 1,600 rpm and at 30° C. for 24 hours, followed by centrifugation to remove the supernatant. To each of the resultants, 0.2 ml of Bugbuster and 0.2 μL of Benzonase Nuclease were added to lyse the cells. The resulting lysates were then centrifuged, and the supernatants were collected. The subsequent operations are the same as those described in the above section 3-1.
It is also noted that, regarding the names of the clones obtained by the method for screening a rabbit-derived single-chain antibody which binds to a human serum-derived IgG polyclonal antibody, the clone of “Clone No. 1 obtained at the completion of Round 1”, for example, is sometimes referred to as “R1-1” or “I-1” in abbreviation. In the same manner, the clone of “Clone No. 1 obtained at the completion of Round 2”, for example, is sometimes referred to as “R2-1” or “II-1”, and the clone of “Clone No. 1 obtained at the completion of Round 3” is sometimes referred to as “R3-1” or “III-1”, in abbreviation.
TABLE 4-1
Clone No.
IgG1
IgG3
IgA
R1-1
0.0330
0.0290
0.0330
R1-2
0.0200
0.0150
0.0160
R1-3
3.1470
2.2850
0.0410
R1-4
0.0300
0.0290
0.0250
R1-5
3.1910
3.0870
0.0230
R1-6
3.1740
2.8820
0.0780
R1-7
3.1240
0.0660
0.0360
R1-8
0.1010
0.1200
0.1200
R1-9
3.1220
2.2560
0.0200
R1-10
2.8020
1.2220
0.0360
R1-11
3.1100
2.9800
0.0480
R1-12
0.0350
0.0230
0.0140
R1-13
3.1020
2.9500
0.0200
R1-14
3.1160
3.0010
0.0220
R1-15
0.0170
0.0130
0.0360
R1-16
0.0310
0.0240
0.0240
R1-17
0.0220
0.0200
0.0230
R1-18
0.0160
0.0090
0.0120
R1-19
0.0110
0.0100
0.0090
R1-20
2.8940
1.0570
0.0190
R1-21
0.0270
0.0150
0.0450
R1-22
0.1530
0.1110
0.1040
R1-23
3.0390
0.8750
0.0170
R1-24
3.0480
0.0530
0.0270
R1-25
3.1200
0.7990
0.0310
R1-26
3.0350
3.0000
0.0200
R1-27
3.0730
3.0820
0.0290
R1-28
0.0170
0.0100
0.0140
R1-29
3.0530
2.2800
0.0530
R1-30
0.0190
0.0170
0.0290
R1-31
0.0360
0.0300
0.0340
R1-32
0.1900
0.1350
0.1150
R1-33
0.0170
0.0180
0.0170
R1-34
3.1380
0.6290
0.0250
R1-35
3.0660
0.5400
0.0170
R1-36
3.1030
0.7110
0.0310
R1-37
0.0080
0.0080
0.0120
R1-38
3.0930
2.9980
0.0210
R1-39
2.9170
0.2600
0.0170
R1-40
0.0330
0.0330
0.0320
R1-41
3.1450
2.1250
0.3290
R1-42
3.1050
2.5150
0.0170
R1-43
3.0910
2.9530
0.0200
R1-44
0.0090
0.0060
0.0120
R1-45
3.0720
2.5140
0.0130
R1-46
0.0080
0.0070
0.0130
R1-47
3.1160
2.8050
0.0190
R1-48
3.1370
2.9600
0.0290
Library
2.9090
1.6280
0.0710
TABLE 4-2
IgG1
IgG3
IgA
Number of positive clones
30
28
4
Number of negative clones
18
20
44
The ratio of the number of
62.5
58.3
8.3
positive clones with respect
to the total 48 clones (%)
OD ≥ 2.5
27
13
0
1 ≤ OD < 2.5
0
6
0
0.1 ≤ OD < 1
3
9
4
In the same manner as above,
TABLE 5-1
Clone No.
IgG1
IgG3
IgA
R2-1
3.1060
2.9480
0.0250
R2-2
3.0650
2.9030
0.0370
R2-3
2.5150
2.5170
0.0100
R2-4
0.0490
0.0630
0.0160
R2-5
2.9640
0.1920
0.0130
R2-6
1.6750
0.2710
0.0120
R2-7
0.0090
0.0090
0.0140
R2-8
3.1140
2.0550
0.0190
R2-9
3.1330
3.0210
0.0200
R2-10
3.1010
2.8040
0.0210
R2-11
2.7430
0.0210
0.0180
R2-12
0.3590
0.0300
0.0150
R2-13
1.4750
0.0130
0.0170
R2-14
2.9970
0.5070
0.0220
R2-15
3.1040
2.9740
0.0200
R2-16
3.1150
3.0470
0.0260
R2-17
3.1850
0.4590
0.0350
R2-18
3.1140
3.0750
3.1080
R2-19
2.7350
1.8010
0.0210
R2-20
2.8910
0.0680
0.0190
R2-21
1.9870
0.2040
0.0160
R2-22
3.1160
0.0400
0.0250
R2-23
2.8150
0.5180
0.0220
R2-24
3.1600
3.1080
0.0380
R2-25
3.1110
2.5610
0.0270
R2-26
3.0630
1.2730
0.0180
R2-27
3.0220
2.4760
0.1570
R2-28
0.8610
1.3530
0.0210
R2-29
0.6900
0.0170
0.0180
R2-30
3.0180
3.0400
0.0210
R2-31
3.1040
2.5360
0.0220
R2-32
3.0850
3.1180
0.0470
R2-33
3.1310
2.8100
0.0240
R2-34
3.1600
1.8090
0.0360
R2-35
3.0810
2.9710
0.0200
R2-36
3.0860
3.0690
0.0310
R2-37
3.0820
2.3490
0.0170
R2-38
3.0670
2.6320
0.0180
R2-39
0.0170
0.0110
0.0150
R2-40
3.1540
2.6190
0.0200
R2-41
3.1320
2.7460
0.0300
R2-42
3.1680
1.7200
0.0210
R2-43
3.1190
1.7940
0.0200
R2-44
3.1840
1.0250
0.0830
R2-45
3.1430
2.8320
0.0180
R2-46
3.1590
1.2460
0.0180
R2-47
3.1440
3.0400
0.0420
R2-48
3.1430
3.1320
0.0260
Library
3.1130
3.0780
1.4940
TABLE 5-2
IgG1
IgG3
IgA
Number of positive clones
45
39
2
Number of negative clones
3
9
46
The ratio of the number of
93.8
81.3
4.2
positive clones with respect
to the total 48 clones (%)
OD ≥ 2.5
39
22
1
1 ≤ OD < 2.5
3
11
0
0.1 ≤ OD < 1
3
6
1
In the same manner as above,
TABLE 6-1
Clone No.
IgG
IgG1
IgG2
IgG3
IgG4
IgA
R3-1
0.0310
0.0370
0.0360
0.0180
0.0370
0.0240
R3-2
3.0800
3.1090
3.0940
3.1140
3.1180
0.0590
R3-3
2.8830
2.9510
2.8880
2.9560
2.6520
0.0340
R3-4
2.5980
2.7860
2.7350
1.7970
2.4910
0.0260
R3-5
2.9690
3.0340
3.0400
3.0120
2.9450
0.0280
R3-6
3.0750
3.0610
3.0590
3.0430
3.1060
0.0380
R3-7
3.0980
2.9180
3.0420
3.0640
3.0510
0.0550
R3-8
3.0140
3.0280
3.0250
3.0600
3.0920
3.0630
R3-9
3.1070
3.0960
3.0760
2.8800
3.0170
0.0420
R3-10
3.0930
3.1050
3.1540
2.7160
3.1220
0.0310
R3-11
3.0930
3.0690
3.0950
3.0400
3.0350
0.0280
R3-12
2.2380
2.5210
2.4300
0.6300
1.9520
0.0200
R3-13
2.8830
2.9640
2.9040
1.1880
2.8740
0.0200
R3-14
3.0970
3.0880
3.1320
2.9640
3.1210
0.0280
R3-15
1.2220
1.5330
1.5390
0.0480
1.1510
0.0280
R3-16
3.0640
3.0810
3.0930
1.5460
3.1160
0.0610
R3-17
3.1290
3.1580
3.0970
3.0340
3.1070
0.0650
R3-18
3.0470
3.0680
3.0980
1.9300
3.1070
0.0400
R3-19
3.0610
3.0910
3.1060
3.0340
3.1140
0.0230
R3-20
0.0820
0.1120
0.1160
0.0310
0.0730
0.0180
R3-21
3.0520
3.0760
3.0870
2.6270
3.0640
0.0970
R3-22
2.9310
3.0260
3.0840
1.5340
3.0600
0.0240
R3-23
3.0370
3.0550
3.0560
3.0220
3.0560
0.0440
R3-24
3.0680
3.0780
3.0790
3.0220
3.0820
0.0680
TABLE 6-2
Clone No.
IgG
IgG1
IgG2
IgG3
IgG4
IgA
R3-25
3.1060
3.1460
3.0560
3.1750
3.2120
0.0320
R3-26
3.0960
3.1000
3.0370
3.1440
3.1580
0.0370
R3-27
3.0960
3.1090
3.0770
3.0890
3.1390
0.0220
R3-28
3.1190
3.1290
3.0440
3.0720
3.1380
0.0220
R3-29
2.1340
3.0510
2.9840
0.1170
2.5800
0.0260
R3-30
3.0330
3.0940
3.0100
3.1070
3.0930
0.0300
R3-31
3.0970
3.0660
3.0280
3.0780
3.1250
0.0370
R3-32
3.0950
2.9880
2.9860
3.1500
3.0800
0.0380
R3-33
3.1380
3.1370
3.1400
3.1270
3.1660
0.0260
R3-34
3.0970
3.1190
3.1370
2.9870
3.1430
0.0200
R3-35
3.0740
3.1400
3.1190
3.0850
3.1080
0.0280
R3-36
3.0880
3.1110
3.1020
2.9920
3.1130
0.0180
R3-37
3.0650
3.0820
3.1260
2.1810
3.1020
0.0940
R3-38
2.7950
2.8820
2.7880
1.2760
2.7010
0.0180
R3-39
3.0760
3.0750
3.1010
2.9760
3.0900
0.0190
R3-40
3.0700
3.1080
3.1080
1.7450
3.1040
0.0400
R3-41
3.0470
3.0970
3.1200
3.1280
3.1680
0.0270
R3-42
3.1050
3.1300
3.1430
3.1020
3.1400
0.0200
R3-43
3.0960
3.1390
3.1510
3.0700
3.1530
0.0190
R3-44
3.0560
3.0620
3.1000
3.1210
3.1030
0.0220
R3-45
3.0570
3.0920
3.1290
2.9400
3.1150
0.0160
R3-46
3.0660
3.1220
3.0540
3.0390
3.1270
0.0170
R3-47
0.1210
0.1750
0.1800
0.0630
0.1080
0.0250
R3-48
3.0760
3.1180
3.1320
2.1820
3.1440
0.0200
TABLE 6-3
Clone No.
IgG
IgG1
IgG2
IgG3
IgG4
IgA
R3-49
3.0920
3.0680
3.0740
3.1260
3.2050
0.0330
R3-50
3.0680
3.0770
3.0960
2.1670
3.1910
0.0200
R3-51
3.0400
3.0480
3.0990
3.0520
3.1630
0.0150
R3-52
3.0640
2.9840
3.0860
3.1580
3.1460
0.0220
R3-53
3.0380
3.0300
3.0860
3.1260
3.1210
0.0580
R3-54
3.0390
3.0520
3.0950
3.0980
3.1660
0.0280
R3-55
3.0520
3.0110
3.1080
3.0960
3.1000
0.0150
R3-56
3.0850
3.0440
3.0910
3.1430
3.1590
0.0540
R3-57
3.0850
3.1320
3.0830
3.0730
3.1420
0.1160
R3-58
3.0460
3.1360
3.0790
3.1140
3.1690
0.0300
R3-59
3.0720
3.1590
3.0710
2.9270
3.1420
0.0180
R3-60
3.0310
3.1390
3.0440
2.9530
3.1010
0.0350
R3-61
3.0360
3.0780
3.0130
3.0230
3.0780
0.0320
R3-62
3.0580
3.0910
3.0490
3.0700
3.1060
0.0320
R3-63
3.0300
3.0620
3.0450
2.9870
3.1170
0.0240
R3-64
3.0750
3.1320
3.0800
2.8780
3.1220
0.0220
R3-65
3.1030
3.0710
3.0540
3.1120
3.1280
0.0270
R3-66
3.0640
3.1340
3.0810
3.0090
3.1370
0.0230
R3-67
3.0520
3.0990
3.0780
2.6830
3.1160
0.0780
R3-68
3.0610
3.0780
3.0630
3.0960
3.0890
0.0760
R3-69
3.0400
3.0640
3.0600
3.0720
3.0470
0.0360
R3-70
3.0430
3.0990
3.0800
3.0040
3.0960
0.0300
R3-71
3.0520
3.0930
3.0790
3.0600
3.0980
0.0170
R3-72
3.0610
3.0880
3.0630
3.0740
3.1290
0.0340
TABLE 6-4
Clone No.
IgG
IgG1
IgG2
IgG3
IgG4
IgA
R3-73
3.0550
3.1000
3.0920
3.1200
3.1370
0.1650
R3-74
3.0070
3.0470
3.0610
3.0800
3.1430
0.0250
R3-75
3.0110
3.0500
3.0400
3.1240
3.1070
3.0610
R3-76
2.9820
3.0840
3.0820
1.2550
3.1270
0.0490
R3-77
3.0360
3.0540
3.0300
3.0740
3.1430
0.0280
R3-78
3.0060
3.0580
3.0560
2.8450
3.0970
0.0300
R3-79
3.0070
3.0510
3.0490
3.0620
3.1290
0.0280
R3-80
3.0410
3.0570
3.0630
2.9360
3.1410
0.0230
R3-81
3.0990
3.1640
3.1200
3.0440
3.1530
0.0410
R3-82
3.0570
3.1510
3.1250
2.6310
3.1620
0.0270
R3-83
3.1000
3.1090
3.1050
2.9730
3.1160
0.0570
R3-84
3.0610
3.1290
3.0800
2.9890
3.1080
0.0930
R3-85
3.0390
3.1480
3.0880
2.9480
3.0770
0.0270
R3-86
2.8250
3.0800
3.0730
0.1340
3.0630
0.0540
R3-87
3.0220
3.1040
3.0650
1.6500
3.0650
0.0210
R3-88
3.0200
3.1380
3.0920
1.8170
3.0970
0.0430
R3-89
2.9340
3.1590
3.1150
1.3950
3.1080
0.0170
R3-90
3.0200
3.1280
3.1080
2.9950
3.1010
0.0240
R3-91
3.0580
3.1570
3.0490
2.9740
3.1160
0.0280
R3-92
3.0360
3.0980
3.0980
2.9290
3.0950
0.0280
R3-93
3.0100
3.1110
3.0990
1.8240
3.0700
0.0470
R3-94
3.0280
3.0970
3.0310
3.0530
3.0950
0.0400
R3-95
3.0360
3.1210
3.1000
2.9770
3.0560
0.0230
R3-96
3.0810
3.1460
3.0000
3.0610
3.1210
0.0250
TABLE 6-5
IgG
IgG1
IgG2
IgG3
IgG4
IgA
Number of positive clones
94
95
95
92
94
4
Number of negative clones
2
1
1
4
2
92
The ratio of the number of
97.9
99
99
95.8
97.9
4.2
positive clones with respect
to the total 96 clones (%)
OD ≥ 2.5
90
92
91
74
90
2
1 ≤ OD < 2.5
3
1
2
15
3
0
0.1 ≤ OD < 1
1
2
2
3
1
2
The above results revealed as follows.
The use of the human serum-derived IgG polyclonal antibody-immobilized MLVs enabled to efficiently collect the phages which bind extremely specifically to the human serum-derived IgG polyclonal antibodies. It is to be noted here that the ratios of the number of positive clones with respect to the total number of the clones exceeded 50% by performing just one round of panning, and such a result is extremely rare, and difficult to achieve with a conventional technique. Further, since the number of positive clones and the amount of binding for each antibody are both markedly increased as the number of rounds performed increases, it can be said that the screening method according to the present invention which uses multilamellar liposomes is an extremely efficient screening technique.
In addition, many of the isolated rabbit-derived single-chain antibodies had a binding specificity for two or more selected from the group consisting of the human IgG1 antibody, the human IgG2 antibody, the human IgG3 antibody, and the human IgG4 antibody. In particular, it is considered that the rabbit-derived single-chain antibodies in which the amounts of binding for the human IgG1 antibody and the human IgG3 antibody are the same, have a high possibility of serving as an affinity ligand which could replace Protein A.
Moreover, although not many in numbers, some of the rabbit-derived single-chain antibodies showed an approximately the same level of absorbance for the human IgA, as the absorbances for the human IgG1 antibody, the human IgG2 antibody, the human IgG3 antibody, and the human IgG4 antibody. This result is thought to suggest that these single-chain antibodies bind specifically to the L chains of the antibodies.
<4. Measurement of Dissociation Rate Constant koff>
Among the 48 colonies collected at the completion of Round 1, the 48 colonies collected at the completion of Round 2, and the 96 colonies collected at the completion of Round 3, the colonies which showed an absorbance exceeding 2.5 in the “Evaluation of Antigen-binding Activity 2” were selected; and the measurement of the dissociation rate constant koff was performed for each of the selected colonies, using Biacore X-100 (manufactured by GE Healthcare Inc.).
(Sample Preparation)
Each of the colonies of the phagemid-containing Escherichia coli cells was inoculated in a well of a 96-well deep well plate, in 1 ml of Overnight Express (registered trademark; manufactured by Merck KGaA) medium, and cultured at 1,600 rpm and at 30° C. for 24 hours, followed by centrifugation to remove the supernatant. To each of the resultants, 0.2 ml of Bugbuster and 0.2 μL of Benzonase Nuclease were added to lyse the cells. The resulting lysates were then centrifuged, and the supernatants were collected. The collected supernatants were each diluted 10-fold with PBST.
(Measuring Method)
The measurement was carried out under the following measurement conditions.
Sensor Chip: human IgG-coupled CM5 (15000 RU)
Running buffer: PBST
Binding time: 300 sec
Dissociation time: 180 sec
Elution: 10 mM Glycine, pH 1.5
According to the method for calculating the dissociation rate constant koff as previously described, the calculations of the dissociation rate constant koff were performed. The calculated results were ranked in the order of descending dissociation rate constant koff values, from Rank 1 to Rank 140, and the results are shown in Table 7-1 to Table 7-5.
TABLE 7-1
Rank
Clone No.
koff (s{circumflex over ( )}−1)
IgG1
IgG3
IgA
1
R3-75
2.78E−04
3.0500
3.1240
3.0610
2
R3-23
4.08E−04
3.0550
3.0220
0.0440
3
R3-26
5.71E−04
3.1000
3.1440
0.0370
4
R3-43
6.41E−04
3.1390
3.0700
0.0190
5
R3-58
7.42E−04
3.1360
3.1140
0.0300
6
R2-18
8.00E−04
3.1140
3.0750
3.1080
7
R2-16
8.38E−04
3.1150
3.0470
0.0260
8
R1-27
8.59E−04
3.0730
3.0820
0.0290
9
R3-42
8.62E−04
3.1300
3.1020
0.0200
10
R3-44
8.74E−04
3.0620
3.1210
0.0220
11
R3-8
8.80E−04
3.0280
3.0600
3.0630
12
R3-24
8.80E−04
3.0780
3.0220
0.0680
13
R3-2
8.97E−04
3.1090
3.1140
0.0590
14
R3-74
9.32E−04
3.0470
3.0800
0.0250
15
R3-25
9.40E−04
3.1460
3.1750
0.0320
16
R3-33
9.42E−04
3.1370
3.1270
0.0260
17
R3-31
9.55E−04
3.0660
3.0780
0.0370
18
R3-28
9.60E−04
3.1290
3.0720
0.0220
19
R3-41
9.71E−04
3.0970
3.1280
0.0270
20
R3-52
9.73E−04
2.9840
3.1580
0.0220
21
R3-54
1.00E−03
3.0520
3.0980
0.0280
22
R3-62
1.05E−03
3.0910
3.0700
0.0320
23
R3-78
1.07E−03
3.0580
2.8450
0.0300
24
R3-59
1.08E−03
3.1590
2.9270
0.0180
25
R3-5
1.11E−03
3.0340
3.0120
0.0280
26
R3-92
1.11E−03
3.0980
2.9290
0.0280
27
R3-56
1.12E−03
3.0440
3.1430
0.0540
28
R3-61
1.13E−03
3.0780
3.0230
0.0320
29
R3-77
1.13E−03
3.0540
3.0740
0.0280
30
R3-6
1.21E−03
3.0610
3.0430
0.0380
TABLE 7-2
Rank
Clone No.
koff (s{circumflex over ( )}−1)
IgG1
IgG3
IgA
31
R3-68
1.22E−03
3.0780
3.0960
0.0760
32
R3-64
1.24E−03
3.1320
2.8780
0.0220
33
R2-3
1.25E−03
2.5150
2.5170
0.0100
34
R3-3
1.27E−03
2.9510
2.9560
0.0340
35
R3-7
1.32E−03
2.9180
3.0640
0.0550
36
R3-85
1.34E−03
3.1480
2.9480
0.0270
37
R3-32
1.34E−03
2.9880
3.1500
0.0380
38
R3-39
1.36E−03
3.0750
2.9760
0.0190
39
R3-34
1.39E−03
3.1190
2.9870
0.0200
40
R2-32
1.39E−03
3.0850
3.1180
0.0470
41
R3-95
1.40E−03
3.1210
2.9770
0.0230
42
R3-21
1.41E−03
3.0760
2.6270
0.0970
43
R2-1
1.42E−03
3.1060
2.9480
0.0250
44
R3-73
1.42E−03
3.1000
3.1200
0.1650
45
R3-46
1.48E−03
3.1220
3.0390
0.0170
46
R2-24
1.49E−03
3.1600
3.1080
0.0380
47
R3-90
1.51E−03
3.1280
2.9950
0.0240
48
R3-91
1.52E−03
3.1570
2.9740
0.0280
49
R3-60
1.52E−03
3.1390
2.9530
0.0350
50
R3-80
1.53E−03
3.0570
2.9360
0.0230
51
R3-82
1.54E−03
3.1510
2.6310
0.0270
52
R2-25
1.57E−03
3.1110
2.5610
0.0270
53
R3-84
1.57E−03
3.1290
2.9890
0.0930
54
R1-43
1.60E−03
3.0910
2.9530
0.0200
55
R3-63
1.62E−03
3.0620
2.9870
0.0240
56
R3-51
1.63E−03
3.0480
3.0520
0.0150
57
R2-31
1.64E−03
3.1040
2.5360
0.0220
58
R3-27
1.64E−03
3.1090
3.0890
0.0220
59
R3-55
1.65E−03
3.0110
3.0960
0.0150
60
R1-5
1.66E−03
3.1910
3.0870
0.0230
TABLE 7-3
Rank
Clone No.
koff (s{circumflex over ( )}−1)
IgG1
IgG3
IgA
61
R3-49
1.67E−03
3.0680
3.1260
0.0330
62
R3-83
1.68E−03
3.1090
2.9730
0.0570
63
R3-45
1.69E−03
3.0920
2.9400
0.0160
64
R3-14
1.71E−03
3.0880
2.9640
0.0280
65
R3-65
1.73E−03
3.0710
3.1120
0.0270
66
R3-36
1.73E−03
3.1110
2.9920
0.0180
67
R3-94
1.74E−03
3.0970
3.0530
0.0400
68
R1-7
1.75E−03
3.1240
0.0660
0.0360
69
R3-9
1.76E−03
3.0960
2.8800
0.0420
70
R2-22
1.86E−03
3.1160
0.0400
0.0250
71
R3-67
1.86E−03
3.0990
2.6830
0.0780
72
R3-96
1.86E−03
3.1460
3.0610
0.0250
73
R2-33
1.86E−03
3.1310
2.8100
0.0240
74
R1-36
1.87E−03
3.0660
0.5400
0.0170
75
R3-70
1.87E−03
3.0990
3.0040
0.0300
76
R3-53
1.88E−03
3.0300
3.1260
0.0580
77
R3-81
1.93E−03
3.1640
3.0440
0.0410
78
R3-17
1.94E−03
3.1580
3.0340
0.0650
79
R3-71
1.94E−03
3.0930
3.0600
0.0170
80
R3-57
1.95E−03
3.1320
3.0730
0.1160
81
R3-30
1.97E−03
3.0940
3.1070
0.0300
82
R2-14
2.04E−03
2.9970
0.5070
0.0220
83
R2-26
2.05E−03
3.0630
1.2730
0.0180
84
R3-79
2.06E−03
3.0510
3.0620
0.0280
85
R1-29
2.08E−03
3.0530
2.2800
0.0530
86
R2-15
2.09E−03
3.1040
2.9740
0.0200
87
R3-19
2.10E−03
3.0910
3.0340
0.0230
88
R2-10
2.11E−03
3.1010
2.8040
0.0210
89
R1-42
2.11E−03
3.1050
2.5150
0.0170
90
R3-11
2.18E−03
3.0690
3.0400
0.0280
TABLE 7-4
Rank
Clone No.
koff (s{circumflex over ( )}−1)
IgG1
IgG3
IgA
91
R1-38
2.22E−03
3.0930
2.9980
0.0210
92
R2-8
2.22E−03
3.1140
2.0550
0.0190
93
R1-39
2.22E−03
2.9170
0.2600
0.0170
94
R2-27
2.28E−03
3.0220
2.4760
0.1570
95
R2-30
2.31E−03
3.0180
3.0400
0.0210
96
R2-5
2.33E−03
2.9640
0.1920
0.0130
97
R1-25
2.33E−03
3.1200
0.7990
0.0310
98
R2-23
2.36E−03
2.8150
0.5180
0.0220
99
R2-34
2.36E−03
3.1600
1.8090
0.0360
100
R3-10
2.38E−03
3.1050
2.7160
0.0310
101
R3-66
2.42E−03
3.1340
3.0090
0.0230
102
R1-47
2.44E−03
3.1160
2.8050
0.0190
103
R3-72
2.44E−03
3.0880
3.0740
0.0340
104
R2-9
2.44E−03
3.1330
3.0210
0.0200
105
R1-13
2.47E−03
3.1020
2.9500
0.0200
106
R1-23
2.48E−03
3.0390
0.8750
0.0170
107
R1-41
2.48E−03
3.1450
2.1250
0.3290
108
R2-35
2.48E−03
3.0810
2.9710
0.0200
109
R3-35
2.53E−03
3.1400
3.0850
0.0280
110
R1-6
2.53E−03
3.1740
2.8820
0.0780
111
R2-17
2.55E−03
3.1850
0.4590
0.0350
112
R3-69
2.59E−03
3.0640
3.0720
0.0360
113
R1-35
2.60E−03
3.1030
0.7110
0.0310
114
R2-37
2.60E−03
3.0820
2.3490
0.0170
115
R1-9
2.65E−03
3.1220
2.2560
0.0200
116
R2-19
2.67E−03
2.7350
1.8010
0.0210
117
R1-24
2.68E−03
3.0480
0.0530
0.0270
118
R2-2
2.82E−03
3.0650
2.9030
0.0370
119
R1-3
2.85E−03
3.1470
2.2850
0.0410
120
R1-20
2.86E−03
2.8940
1.0570
0.0190
TABLE 7-5
Rank
Clone No.
koff (s{circumflex over ( )}−1)
IgG1
IgG3
IgA
121
R2-11
2.96E−03
2.7430
0.0210
0.0180
122
R2-45
3.09E−03
3.1430
2.8320
0.0180
123
R2-48
3.14E−03
3.1430
3.1320
0.0260
124
R1-34
3.27E−03
3.1380
0.6290
0.0250
125
R1-48
3.45E−03
3.1370
2.9600
0.0290
126
R1-45
3.47E−03
3.0720
2.5140
0.0130
127
R1-26
3.63E−03
3.0350
3.0000
0.0200
128
R1-14
3.66E−03
3.1160
3.0010
0.0220
129
R2-42
3.87E−03
3.1680
1.7200
0.0210
130
R1-10
4.00E−03
2.8020
1.2220
0.0360
131
R2-44
4.06E−03
3.1840
1.0250
0.0830
132
R2-47
4.11E−03
3.1440
3.0400
0.0420
133
R1-11
4.38E−03
3.1100
2.9800
0.0480
134
R2-40
4.88E−03
3.1540
2.6190
0.0200
135
R2-46
6.78E−03
3.1590
1.2460
0.0180
136
R2-41
6.94E−03
3.1320
2.7460
0.0300
137
R2-43
6.95E−03
3.1190
1.7940
0.0200
138
R2-38
9.89E−03
3.0670
2.6320
0.0180
139
R2-20
Unmeasurable
2.8910
0.0680
0.0190
140
R2-36
Unmeasurable
3.0860
3.0690
0.0310
<5. Determination of Amino Acid Sequences of Genes of Rabbit-Derived Single-Chain Antibodies which Bind to Human Serum-Derived IgG Polyclonal Antibodies>
For the clones which had been ranked as Rank 1 (R3-75), Rank 2 (R3-23), Rank 3 (R3-26), Rank 4 (R3-43), Rank 5 (R3-58), Rank 6 (R2-18), Rank 7 (R2-16), Rank 8 (R1-27), Rank 11 (R3-8), and Rank 68 (R1-7) based on the measurement results of the dissociation rate constant koff, the amino acid sequences were determined from the gene sequences of the rabbit-derived single-chain antibody genes. The clone ranked as Rank 4 (R3-43) could not be sequenced.
Further, regarding the genes of the variable regions (VL domains) of the light chains (L chains) shown in
The rabbit-derived single-chain antibody genes obtained from Rank 1 (R3-75), Rank 6 (R2-18), and Rank 11 (R3-8) were found to contain the sequence “ATRYDSYGYAYNYWFGTLW (SEQ ID NO: 30, 19 residues)” as CDR3. The rabbit-derived single-chain antibodies derived from these colonies are those which bind to the human IgG1 antibody, the human IgG2 antibody, the human IgG3 antibody, the human IgG4 antibody, and the human IgA antibody.
The rabbit-derived single-chain antibody gene obtained from Rank 2 (R3-23) was found to contain the sequence “GSYYDSHGYAYVSLW (SEQ ID NO: 31, 15 residues)” as CDR3. The rabbit-derived single-chain antibody obtained from this colony is one which binds to the human IgG1 antibody, the human IgG2 antibody, the human IgG3 antibody, and the human IgG4 antibody.
The rabbit-derived single-chain antibody gene obtained from Rank 3 (R3-26) was found to contain the sequence “ATDYGIYGYAYGHLW (SEQ ID NO: 32, 15 residues)” as CDR3. The rabbit-derived single-chain antibody obtained from this colony is one which binds to the human IgG1 antibody, the human IgG2 antibody, the human IgG3 antibody, and the human IgG4 antibody.
The rabbit-derived single-chain antibody genes obtained from Rank 5 (R3-58) and Rank 8 (R1-27) were found to contain the sequence “ARYSGDNGGTLNLW (SEQ ID NO: 33, 14 residues)” as CDR3. The rabbit-derived single-chain antibodies obtained from these colonies are those which bind to the human IgG1 antibody, the human IgG2 antibody, the human IgG3 antibody, and the human IgG4 antibody.
The rabbit-derived single-chain antibody gene obtained from Rank 7 (R2-16) was found to contain the sequence “ARYSGDNGGALNLW (SEQ ID NO: 34, 14 residues)” as CDR3. The rabbit-derived single-chain antibody obtained from this colony is one which binds to the human IgG1 antibody, the human IgG2 antibody, the human IgG3 antibody, and the human IgG4 antibody.
<6. Measurement of Binding Capacity for Human IgG1 Antibody>
The binding capacity for the human IgG1 antibody was measured, for each of the rabbit-derived single-chain antibodies obtained from the colonies which had been ranked as Rank 1 (R3-75), Rank 2 (R3-23), Rank 6 (R2-18), Rank 7 (R2-16), Rank 8 (R1-27), and Rank 68 (R1-7) based on the measurement results of the dissociation rate constant koff, using Biacore X-100 (manufactured by GE Healthcare Inc.).
(Sample Preparation Method)
Each of the collected colonies of the phagemid-containing Escherichia coli cells was inoculated in a 500-ml flask equipped with a baffle, in 50 ml of Overnight Express (registered trademark; manufactured by Merck KGaA) medium, and cultured at 30° C. and at 200 rpm for 24 hours, followed by centrifugation to remove the supernatant. To each of the resultants, 5 ml of Bugbuster and 0.2 μL of Benzonase Nuclease were added to lyse the cells. The resulting lysates were then centrifuged, and the supernatants were collected. The supernatants were each diluted 10-fold with PBST, to be used as measurement samples.
(Measuring Method)
The measurement was carried out under the following measurement conditions.
Sensor Chip: human IgG1-coupled CM5 (5000 RU)
Running buffer: PBST
Binding time: 540 sec
Dissociation time: 120 sec
Elution: 10 mM Glycine, pH 1.5
The same procedure as in Example 6 was carried out as Comparative Example 6-1, except that Protein A (29435-14; manufactured by Nakalai Tesque, Inc.) prepared with PBST to a final concentration of 10 g/mL was used, instead of the sample.
The same procedure as in Example 6 was carried out as Comparative Example 6-2, except that a mouse scFv-FM (soluble fraction was diluted 10-fold with PBST) was used, instead of the sample.
The obtained colony of the phagemid-containing Escherichia coli cells was inoculated in a 500-ml flask equipped with a baffle, in 50 ml of Overnight Express (registered trademark; manufactured by Merck KGaA) medium, and cultured at 30° C. and at 200 rpm for 24 hours, followed by centrifugation to remove the supernatant. To the resultant, 5 ml of Bugbuster and 0.2 μL of Benzonase Nuclease were added to lyse the cells. The resulting lysate was then centrifuged, and the supernatant was collected. The supernatant was diluted 10-fold with PBST, and used in the measurement.
Measurement results are shown in
<7. Measurement of Dissociation Constant KD for Human IgG1 Antibody>
The dissociation constant KD for the human IgG1 antibody was measured, for each of the rabbit-derived single-chain antibodies obtained from the colonies which had been ranked as Rank 1 (R3-75), Rank 2 (R3-23), Rank 3 (R3-26), Rank 6 (R2-18), Rank 7 (R2-16), Rank 8 (R1-27), and Rank 68 (R1-7) based on the measurement results of the dissociation rate constant koff, using Biacore X-100 (manufactured by GE Healthcare Inc.).
(Sample Preparation Method)
A DNA fragment containing the rabbit-derived single-chain antibody gene was amplified by PCR from the phagemid vector of each colony, using T7 promoter primer and M13 primer. After purification, the DNA fragment was digested with restriction enzymes Xba I and Not I, and inserted into the Xba I/Not I sites of a pET22 vector (manufactured by Merck KGaA). The thus constructed rabbit-derived single-chain antibody expression vector allows the rabbit-derived single-chain antibody to be expressed in the form in which a pelB leader signal sequence is fused to the N-terminus, and a histidine tag (6×His-tag) is fused to the C-terminus. After the expression, the rabbit-derived single-chain antibody migrates to the periplasm and the pelB leader sequence is cleaved by a signal peptidase.
The thus constructed rabbit-derived single-chain antibody-His expression vector was used to transform Escherichia coli Rosetta (DE3) cells, and the transformed cells were cultured on an LB agar plate (containing 50 mg/L ampicillin and 35 mg/L kanamycin). The resulting single colony was cultured overnight in 10 ml of an LB medium (containing 50 mg/L ampicillin and 35 mg/L kanamycin). The obtained culture liquid was inoculated in 50 ml of Overnight Express TB medium (manufactured by Merck KGaA) and cultured at 37° C. and at 200 rpm for 24 hours.
The resulting culture liquid was centrifuged (10,000 rpm, 4° C., 15 minutes), and the culture supernatant was obtained. Further, the cells were suspended in 5 ml of lysis buffer containing Bugbuster, lysozyme, and Benzonase Nuclease, and incubated at 37° C. for one hour to lyse the cells. Following centrifugation at 10,000 rpm and at 4° C. for 15 minutes, the supernatant was collected as the intracellular soluble fraction.
The above described culture supernatant and the intracellular soluble fraction were each applied to a His-Trap HP column (manufactured by GE Healthcare), and subjected to a gradient elution using 0.4 M imidazole, to collect the rabbit-derived single-chain antibody-His. For each of the obtained eluants, the protein concentration was quantified by DC Protein assay (Biorad). Further, the purity of the rabbit-derived single-chain antibody-His in each eluant was confirmed by SDS-PAGE. When the purity of the rabbit-derived single-chain antibody-His in the eluant was not sufficient, the eluant was further purified by a human IgG-coupled column, and then quantified. The collected eluants were each diluted 10-fold or more with PBST, and the measurement of the dissociation constant KD was carried out using Biacore X-100.
(Measuring Method)
The measurement was carried out under the following measurement conditions.
Sensor Chip: human IgG1-coupled CM5 (5000 RU)
Running buffer: PBST
Binding time: 180 sec
Dissociation time: 600 sec
Elution: 10 mM Glycine, pH 1.5
Mode: Single cycle kinetics mode
The properties of the thus obtained rabbit-derived single-chain antibodies, including the measurement results of the dissociation constant KD, are summarized in Table 8. The dissociation constant KD of the rabbit-derived single-chain antibody of Rank 1 (R3-75) for the human IgG1 antibody was found out to be 5.5×10−10 M. In view of the fact that the dissociation constant KD of Protein A for the human IgG1 antibody is around 5 to 10 nM, the rabbit-derived single-chain antibody of Rank 1 (R3-75) is thought to bind extremely strongly to the human IgG1 antibody.
Further, in the column “Location” in Table 8, one whose activity was confirmed using a sample of culture supernatant is indicated as “Supernatant”, and one whose activity was confirmed using a sample of soluble fraction is indicated as “Periplasm”. When indicated as “Supernatant”, it means that the phage or rabbit-derived single-chain antibody was secreted from the Escherichia coli, and when indicated as “Periplasm”, it means that the phage or rabbit-derived single-chain antibody was present in the periplasm of Escherichia coli.
[Table 8]
TABLE 8
Clone
kon
koff
Rmax
Rank
No.
(M−1s−1)
(s−1)
KD (M)
(RU)
Location
1
R3-75
6.7 × 104
3.7 × 10−5
5.5 × 10−10
342.2
Super-
natant
2
R3-23
1.1 × 104
1.3 × 10−4
1.1 × 10−8
364.1
Periplasm
3
R3-26
2.1 × 104
4.3 × 10−5
2.1 × 10−9
329.4
Super-
natant
6
R2-18
2.5 × 104
1.2 × 10−4
4.8 × 10−9
364.1
Super-
natant
7
R2-16
1.3 × 105
3.2 × 10−4
2.5 × 10−9
241.8
Periplasm
8
R1-27
9.9 × 103
4.0 × 10−4
4.0 × 10−8
530.6
Periplasm
68
R1-07
7.1 × 104
1.7 × 10−3
2.4 × 10−8
79.9
Periplasm
The rabbit-derived single-chain antibodies of Rank 1 (R3-75), Rank 3 (R3-26), and Rank 6 (R2-18) were found to be secreted in the culture supernatant.
<8. Separation Agent for Separating Human Serum-Derived IgG Polyclonal Antibody>
(Preparation of Single-Chain Antibody)
The single-chain antibody of “R3-26” was mass produced, by fed-batch culture using a Jar Fermenter. Further, the single-chain antibody secreted in the culture supernatant was purified using a HisTrap HP column (manufactured by GE Healthcare Inc.) by immobilized metal ion affinity chromatography (IMAC). Further, a Hi Trap Desalting column (manufactured by GE Healthcare Inc.) for desalting and buffer replacement was used to replace the buffer with 0.1 M carbonate buffer (pH 8.3) containing 0.5 M NaCl, and then concentrated by ultrafiltration. Finally, the single-chain antibody having a concentration of 1 mg/ml and a volume of 10 ml was obtained.
(Immobilization of Single-Chain Antibody on Carrier)
The carboxyl group of Sepharose (agarose carrier in the form of beads), which is the carrier in a 5 ml HiTrap NHS column (manufactured by GE Healthcare Inc.), was esterified with NHS, and the purified single-chain antibody described above was supplied to the column so that an amino group of the single-chain antibody forms an amide bond with the carboxyl group, thereby immobilizing the single-chain antibody on the column. Ethanolamine was added to the column to block the unreacted NHS esters.
(Separation of Human Serum-Derived IgG Polyclonal Antibody)
The 5 ml column on which the single-chain antibody was immobilized was set in a chromatography system, AKTA Purifier UPC 10 (manufactured by GE Healthcare Inc.), and equilibrated with PBS. To the column, 10 ml of a human serum-derived IgG polyclonal antibody (#I4506; manufactured by Sigma-Aldrich Co. LLC.) prepared to a concentration of 1 mg/ml was supplied at a flow velocity of 1 ml/min. Subsequently, the column was washed with PBS. After confirming that the value of UV280 reached the baseline, 0.5 M arginine (pH 1.5) was supplied to the column, to elute the human serum-derived IgG polyclonal antibody from the column.
As a result, the breakthrough curve as shown in
The above results suggested the usability of a single-chain antibody selected by the screening method according to the present invention as a separation agent for separating a human serum-derived IgG polyclonal antibody.
<9. Method for Screening Rabbit-Derived Single-Chain Antibody which Specifically Binds to L Chain of Human Antibody>
The previously examined evaluation results of the antigen specificity and the amino acid sequence, carried out for each of the total 192 clones obtained in Rounds 1 to 3 in the panning using the human serum-derived IgG polyclonal antibody-immobilized MLVs, revealed that 3 clones (R2-18, R3-8, and R3-75) strongly bind not only to the human IgG antibodies, but also to the human IgA antibody.
Further, the analysis of the antigen specificities of these single-chain antibodies by Western blotting revealed that these single-chain antibodies recognize the light chains (L chains), specifically, the kappa chains, of the human antibodies. When the amino acid sequences of the constant regions are compared between a human IgG antibody and a human IgA antibody, the amino acid sequences of the heavy chains (H chains) are completely different between the two. In contrast, the light chains (L chains) are broadly classified into lambda and kappa chains, and the amino acid sequences of the lambda chains are common between IgG and IgA, and so are the amino acid sequences of the kappa chains. This also applies to the case of a human IgM antibody, a human IgE antibody, a human IgD antibody, and the like. Thus, it has been suggested that these 3 clones are antibodies with an extremely high added value, which are capable of specifically binding not only to a human IgG antibody and a human IgA antibody, but also to all types of the human antibodies including a human IgM antibody, a human IgE antibody, a human IgD antibody, and the like.
Therefore, in order to collect such a rabbit-derived single-chain antibody which specifically binds to the L chain of a human antibody, in a highly efficient manner, from the previously prepared library of phages presenting the anti-human serum-derived IgG polyclonal antibody-rabbit-derived single-chain antibodies, the panning as described below was further performed.
A description will be given below regarding the method for screening a rabbit-derived single-chain antibody which specifically binds to the L chain of a human antibody (hereinafter, sometimes referred to as an “anti-human antibody L chain-rabbit-derived single-chain antibody”) from a phage library.
It is noted that, regarding the names of clones obtained by the method for screening an anti-human antibody L chain-rabbit-derived single-chain antibody, the clone of “Clone No. 1 obtained at the completion of Round 1”, for example, is sometimes referred to as “IgA R1-1” or “IgA I-1” in abbreviation. In the same manner, the clone of “Clone No. 1 obtained at the completion of Round 2”, for example, is sometimes referred to as “IgA R2-1” or “IgA II-1”, and the clone of “Clone No. 1 obtained at the completion of Round 3” is sometimes referred to as “IgA R3-1” or “IgA III-1”, in abbreviation.
<9-1. Coupling of Human Serum-Derived IgA Polyclonal Antibody to Multilamellar Liposomes>
Human serum-derived IgA polyclonal antibody-immobilized MLVs were prepared in the same manner as described in the above section 1-1. As the human serum-derived IgA polyclonal antibody, #I4036 manufactured by Sigma-Aldrich Co. LLC. was used.
<9-2. Preparation of Library of Phages Presenting Anti-Human Serum-Derived IgG Polyclonal Antibody-Rabbit-Derived Single-Chain Antibodies>
A library of phages presenting the anti-human serum-derived IgG polyclonal antibody-rabbit-derived single-chain antibodies was prepared, in the same manner as described in the above described section 2-2.
<9-3. Panning>
Panning was carried out in the same manner as in the above 2-3, using the phage library prepared in the above 9-2 and the human serum-derived IgA polyclonal antibody-immobilized MLVs prepared in the above 9-1.
The same procedure as in Example 9-1 was carried out as Comparative Example 9-1, except that multilamellar liposomes on which the human serum-derived IgA polyclonal antibody had not been immobilized were used.
<9-4. Recovery of Phages to Gene Sequencing>
The presence or absence of the genes of anti-human serum-derived IgA polyclonal antibody-rabbit-derived single-chain antibodies was confirmed in the phagemid DNAs recovered in Example 9-1 and Comparative Example 9-1, in the same manner as described in the above described 2-2.
<9-5. Panning Results>
It can be seen from the above results that the recovery rate markedly increased in Round 3 in Example 9-1, to a level not less than 100-times the recovery rate in Comparative Example 9-1. This has confirmed that it is possible to carry out an efficient panning, also in the case of using the human serum-derived IgA polyclonal antibody-immobilized MLVs.
<9-6. Evaluation of Antigen-Binding Activity 1>
In the same manner as in the above section 3-1, the evaluation of the antigen-binding activity was carried out for the rabbit-derived single-chain antibodies obtained from the pellet portion of the phagemid-containing Escherichia coli cells (namely, the entire phages contained in the Escherichia coli cells which did not form single colonies and contained in the pellets) collected in each of the rounds, as follows. Note, however, that the human IgA antibody (#I4036; manufactured by Sigma-Aldrich Co. LLC.) alone was used as the antigen to be immobilized on plates, and the evaluation of the antigen-binding activity was also performed only for the human IgA antibody. In other words, the immobilization of the human IgG1 antibody and the like, and the evaluation of the antigen-binding activity for the human IgG1 antibody and the like, were not carried out.
The results are shown in
<9-7. Evaluation of Antigen-Binding Activity 2>
The evaluation of the antigen-binding activity was carried out for the rabbit-derived single-chain antibodies obtained from the colonies of the phagemid-containing Escherichia coli cells collected in each of the rounds, in the same manner as in the above section 3-2. Note that, in this Example, not only the human IgA antibody (#I4036; manufactured by Sigma-Aldrich Co. LLC.), but also the human IgG 1 antibody and the like were used as the antigens to be immobilized on plates, in the same manner as in the above 3-2. Likewise, the evaluation of the antigen-binding activity was carried out not only for the human IgA antibody, but also for the human IgG 1 antibody and the like.
TABLE 9-1
Clone No
IgG1
IgG2
IgG3
IgG4
IgA
IgA R1-1
0.0850
0.1040
0.2120
0.0440
0.0380
IgA R1-2
0.0600
0.0760
0.0690
0.0280
0.0240
IgA R1-3
0.0540
0.0560
0.0790
0.0270
0.0200
IgA R1-4
0.2200
0.5880
1.5880
0.5000
0.2600
IgA R1-5
0.0600
0.1100
0.6720
0.0970
0.0440
IgA R1-6
0.0500
0.0650
0.0850
0.0330
0.0270
IgA R1-7
0.0730
0.1150
0.9080
0.1290
0.0920
IgA R1-8
0.2330
0.2670
0.6240
0.3280
0.2690
IgA R1-9
0.1810
0.0760
0.1100
0.0300
0.0310
IgA R1-10
0.0270
0.0820
0.2070
0.0440
0.0320
IgA R1-11
0.0180
0.0570
0.0770
0.0250
0.0210
IgA R1-12
0.0220
0.0750
0.1360
0.0350
0.0270
IgA R1-13
0.0190
0.0590
0.1230
0.0340
0.0260
IgA R1-14
0.0450
0.1510
0.9870
0.1680
0.1210
IgA R1-15
0.0220
0.0800
0.0950
0.0350
0.0300
IgA R1-16
0.0520
0.1140
0.2510
0.0670
0.0430
IgA R1-17
0.0240
0.0710
0.3950
0.0580
0.0290
IgA R1-18
0.3240
0.7110
1.8720
0.6230
0.3630
IgA R1-19
0.4750
0.2010
1.3900
2.2470
0.6940
IgA R1-20
0.0390
0.2960
0.2900
0.1420
0.1120
IgA R1-21
0.0120
0.0560
0.0820
0.0210
0.0170
IgA R1-22
0.0830
0.1650
1.6250
0.2780
0.1050
IgA R1-23
0.0200
0.0570
0.1450
0.0310
0.0230
IgA R1-24
0.0460
0.0600
0.0600
0.0190
0.0210
IgA R1-25
0.0210
0.0850
0.3760
0.0490
0.0310
IgA R1-26
0.0330
0.1190
0.3780
0.0790
0.0500
IgA R1-27
0.0630
0.0810
0.6180
0.1260
0.0540
IgA R1-28
0.0490
0.1350
0.6880
0.1000
0.0640
IgA R1-29
0.0320
0.1310
0.8010
0.1050
0.0610
IgA R1-30
0.0130
0.0640
0.1430
0.0280
0.0220
IgA R1-31
0.1870
0.6220
1.8370
0.6150
0.2750
IgA R1-32
1.2300
2.1850
2.7570
2.0930
2.5720
TABLE 9-2
IgG1
IgG2
IgG3
IgG4
IgA
Number of positive clones
7
16
25
13
9
Number of negative clones
25
16
7
19
23
The ratio of the number of
21.9
500
78.1
406
28.1
positive clones to the total
32 clones (%)
OD ≤ 2.5
0
0
1
0
1
1 ≤ OD < 2.5
1
1
5
2
0
0.1 ≤ OD < 1
6
15
19
11
8
Likewise,
TABLE 10-1
Clone No.
IgG1
IgG2
IgG3
IgG4
IgA
IgA R2-1
0.0140
0.0560
0.0710
0.0220
0.0200
IgA R2-2
3.0900
3.0160
2.9940
2.9860
2.9130
IgA R2-3
3.1110
2.9990
2.9910
2.9780
2.9280
IgA R2-4
2.9270
2.9660
2.9890
2.9540
2.9070
IgA R2-5
0.0100
0.0540
0.0760
0.0220
0.0180
IgA R2-6
3.0640
2.9620
2.9640
2.9300
2.8760
IgA R2-7
0.0090
0.0450
0.0270
0.0170
0.0180
IgA R2-8
3.1390
3.0310
3.0200
3.0030
2.9220
IgA R2-9
0.0330
0.0980
0.4670
0.0560
0.0450
IgA R2-10
3.0600
3.0060
3.0150
2.9410
2.8700
IgA R2-11
3.0650
2.9860
2.9960
2.9860
2.8940
IgA R2-12
0.2040
0.4280
2.2810
0.5590
0.2790
IgA R2-13
0.0430
0.1360
1.5570
0.1690
0.0660
IgA R2-14
0.1150
0.3220
1.3980
0.2480
0.1490
IgA R2-15
0.0380
0.1140
0.7580
0.1350
0.0550
IgA R2-16
0.0720
0.1760
1.6820
0.1760
0.0630
IgA R2-17
0.0690
0.1650
1.7400
0.2470
0.1160
IgA R2-18
0.0120
0.0520
0.0850
0.0220
0.0210
IgA R2-19
0.0250
0.0950
0.6030
0.0590
0.0380
IgA R2-20
3.0290
3.0270
2.9720
2.9640
2.8480
IgA R2-21
0.0080
0.0460
0.1020
0.0150
0.0170
IgA R2-22
2.8440
3.0150
2.9650
2.9660
2.8580
IgA R2-23
0.0320
0.1070
1.1400
0.0960
0.0410
IgA R2-24
0.1180
0.5180
1.9500
0.3020
0.4330
IgA R2-25
0.0810
0.2390
1.6760
0.4050
0.1340
IgA R2-26
3.0840
2.9940
2.9820
3.0180
2.9360
IgA R2-27
0.1000
0.4810
1.4420
0.3820
0.2800
IgA R2-28
3.0400
2.9900
2.9300
2.9910
2.9560
IgA R2-29
2.1590
2.8960
2.8920
1.0310
2.7930
IgA R2-30
0.2730
0.6990
1.7850
0.6590
0.4920
IgA R2-31
0.1900
2.4280
1.2270
1.4560
0.0990
IgA R2-32
0.0620
0.1050
0.4250
0.0760
0.0650
TABLE 10-2
IgG1
IgG2
IgG3
IgG4
IgA
Number of positive clones
18
25
28
23
19
Number of negative clones
14
7
4
9
13
The ratio of the number of
56.3
78.1
87.5
71.9
59.4
positive clones to the total
32 clones (%)
OD ≥ 2.5
11
12
12
11
12
1 ≤ OD < 2.5
1
1
11
2
0
0.1 ≤ OD < 1
6
12
5
10
7
Likewise,
TABLE 11-1
Clone No.
IgG1
IgG2
IgG3
IgG4
IgA
IgA R3-1
3.0930
3.0670
3.0240
3.0710
2.9960
IgA R3-2
3.0790
3.0310
2.9910
3.0140
2.9740
IgA R3-3
0.2860
2.7640
2.9480
2.9950
2.8860
IgA R3-4
3.0610
3.0250
2.9770
3.0420
2.9520
IgA R3-5
3.1030
3.0350
2.9900
3.0390
2.9580
IgA R3-6
3.0930
3.0310
2.9770
3.0500
2.9540
IgA R3-7
3.0870
3.0090
2.9810
3.0490
2.9950
IgA R3-8
3.0920
3.0590
3.0440
3.0210
2.9840
IgA R3-9
3.0780
3.0910
3.0370
3.0210
2.9860
IgA R3-10
3.1220
3.0150
3.0140
3.0280
2.9690
IgA R3-11
2.9950
3.0290
2.9600
3.0350
3.0260
IgA R3-12
3.0610
3.0490
2.9380
3.0060
3.0120
IgA R3-13
2.8620
2.9970
2.9940
3.0250
3.0410
IgA R3-14
3.0680
3.0490
2.9530
3.0210
3.0010
IgA R3-15
3.0920
3.0420
2.9610
3.0480
2.9550
IgA R3-16
3.0900
3.0750
3.0210
3.0380
2.9770
IgA R3-17
3.1130
3.0810
2.9750
3.1040
3.0100
IgA R3-18
3.0910
3.0900
2.9910
3.0790
3.0340
IgA R3-19
2.9280
3.0170
2.9810
3.0840
2.9920
IgA R3-20
3.0290
3.0130
2.9810
3.0490
2.9650
IgA R3-21
3.0950
3.0490
2.9920
3.0600
2.9960
IgA R3-22
3.0400
3.0500
2.9610
3.1010
3.0010
IgA R3-23
3.0360
3.0310
2.9540
3.0780
2.9660
IgA R3-24
3.1110
3.0640
2.9940
3.0400
2.9730
IgA R3-25
3.0670
3.1040
2.9840
3.1550
3.0870
IgA R3-26
2.8440
3.0730
3.0000
3.0990
3.0030
IgA R3-27
3.0450
3.0810
3.0150
3.1110
3.0520
IgA R3-28
3.0470
3.0720
3.0050
3.0910
3.0640
IgA R3-29
2.7280
3.0550
2.9890
3.1130
3.0150
IgA R3-30
3.0490
2.9040
2.9910
3.0780
3.1070
IgA R3-31
3.0370
3.0520
2.9900
3.1030
2.9870
IgA R3-32
2.7580
3.0530
2.9610
3.0670
3.0590
TABLE 11-2
IgG1
IgG2
IgG3
IgG4
IgA
Number of positive clones
32
32
32
32
32
Number of negative clones
0
0
0
0
0
The ratio of the number of
100
100
100
100
100
positive clones to the total
32 clones (%)
OD ≥ 2.5
31
32
32
32
32
1 ≤ OD < 2.5
0
0
0
0
0
0.1 ≤ OD < 1
1
0
0
0
0
The above results revealed as follows.
All of the single-chain antibodies collected at Round 3 bound to the human IgA antibody, with an extremely high binding activity. Further, these single-chain antibodies bound not only to the human IgA antibody, but also to all of the human IgG1 antibody, the human IgG2 antibody, the human IgG3 antibody, and the human IgG4 antibody. These results revealed that the panning has been carried out at an extremely high efficiency.
<9-8. Determination of Amino Acid Sequences of Genes of Rabbit-Derived Single-Chain Antibodies which Bind to Human Serum-Derived IgA Polyclonal Antibody>
The amino acid sequences of the rabbit-derived single-chain antibodies obtained from the 32 colonies collected at the completion of Round 1, the 32 colonies collected at the completion of Round 2, and the 32 colonies collected at the completion of Round 3 were determined, from the gene sequences of the rabbit-derived single-chain antibody genes.
Further, for the amino acid sequences of CDR3 of the VH domains, which greatly affect the specificity of the antigen-antibody reaction, the number of amino acid residues, the number of emergence of the sequence in 32 clones, and the probability of emergence in 32 clones are shown for each sequence in
Likewise, the results for the 32 colonies obtained at the at the completion of Round 2 are shown in
Further, the amino acid sequences of the VH domains of “R2-18”, “R3-8” and “R3-75” obtained in the section of <2. Method for Screening Rabbit-derived Single-chain Antibody which Binds to Human Serum-derived IgG Polyclonal Antibody> described above are shown in
Further, a plurality of clones in the FIGS. are indicated with the notation, for example, “Common 1” in the remarks column. This indicates that the clones denoted as “Common 1” are all identical clones. Likewise, the clones denoted as “Common 2” are all identical clones. Note, however, that these numbers are given merely for convenience sake.
Still further, there are clones which are indicated with the notation, for example, “Common 3 (identical to R3-75)”, in the remarks column. This indicates that these clones are identical to the clone “R3-75” obtained in the section of <2. Method for Screening Rabbit-derived Single-chain Antibody which Binds to Human Serum-derived IgG Polyclonal Antibody>.
Further, the numbers of clones of “Common 1” to “Common 7” at the completion of Rounds 1 to 3 are summarized in
The above results revealed as follows.
As can be seen from the results shown in
Among these, 12 clones were clones of Common 1, and 8 clones were clones of Common 2. Two other clones were clones of Common 4, which are identical with “R2-18 (Rank 6; note, however, that this clone is identical to the clone “R3-8”)” obtained in the section of <2. Method for Screening Rabbit-derived Single-chain Antibody which Binds to Human Serum-derived IgG Polyclonal Antibody>.
Further, two other clones were clones of Common 3, which are identical to the clone “R3-75 (Rank 1)” obtained in the section of <2. Method for Screening Rabbit-derived Single-chain Antibody which Binds to Human Serum-derived IgG Polyclonal Antibody>.
In addition, a plurality of clones were also obtained, whose amino acid sequences of CDR3 of the VH domains are highly homologous with each other, such as the sequences “ARADYNTVAYFDLW (SEQ ID NO: 141; 14 residues)”, “ARADYNTAAYFDLW (SEQ ID NO: 142; 14 residues)”, and “VRADYNTVSYFDLW (SEQ ID NO: 143; 14 residues)”.
The results of Western blotting have revealed that all the clones obtained in Round 3 bind to the light chains (L chains) of the human antibodies, specifically to the kappa chains, regardless of the length of the amino acid sequence of the CDR3 of the VH domain.
Based on the above results, it has been found out that, by carrying out panning using a human serum-derived IgA polyclonal antibody as an antigen to be immobilized on a carrier, it is possible to collect a single-chain antibody which binds to the light chain (L chain), specifically to the kappa chain, of a human antibody, which is a region common to both a human IgG antibody and a human IgA antibody, with an extremely high efficiency.
<9-9. Measurement of Dissociation Rate Constant koff>
The measurement of the dissociation rate constant koff was carried out for the 32 colonies obtained at the completion of Round 3, in the same manner as described in the section of <4. Measurement of Dissociation Rate Constant koff> above, except that human IgA antibody immobilized CM5 was used as a sensor chip. These results are shown in
The same procedure as in Example 11 was carried out as Comparative Example 11, except for using “IgA R1-2” as a negative control.
TABLE 12
Clone No.
koff (sec−1)
R2
Remarks
IgA R3-6
8.69E−05
9.92E−01
Common 1
IgA R3-2
1.48E−04
9.92E−01
Common 2
IgA R3-1
9.88E−05
9.81E−01
Common 3
IgA R3-18
1.81E−04
9.93E−01
Common 4
IgA R3-7
9.56E−05
9.74E−01
Common 5
IgA R3-19
9.81E−04
9.84E−01
Common 6
IgA R3-13
1.31E−04
9.95E−01
Common 7
IgA R3-3
6.75E−04
9.53E−01
IgA R3-26
1.00E−03
9.86E−01
IgA R3-29
6.61E−04
9.97E−01
IgA R3-32
5.64E−04
9.99E−01
IgA R1-2
—
—
It has been confirmed that all the clones obtained in Round 3 bind to the human IgA antibody. Further, as shown in Table 12, the most of the single-chain antibodies derived from the clones obtained in Round 3 had a dissociation rate constant koff within the order of from 10−5 to 10−4 sec−1, which is extremely low. In particular, the dissociation rate constant koff of the single-chain antibody derived from “IgA R3-6 (Common 1)”, which accounted for 12 clones out of 32 clones, was lower than the dissociation rate constant koff of the single-chain antibody derived from “IgA R3-1 (Common 3)”, which is identical to the clone R3-75”, suggesting a high affinity of the single-chain antibody derived from “IgA R3-6 (Common 1)”.
Based on the above results, it has been found out that the present method is also capable of collecting a clone which is present at a low abundance in the library, at an extremely high efficiency, and is effective for collecting a single-chain antibody having a high affinity and specificity.
The present invention can be used, for example, in a method for producing an antibody drug.
Hasegawa, Yuya, Uchimura, Seiichi, Kumada, Yoichi
Patent | Priority | Assignee | Title |
Patent | Priority | Assignee | Title |
4618589, | Jul 16 1980 | THE UNIVERSITY OF BIRMINGHAM | Immunoprecipitation assay of immunoglobulins using monoclonal antibodies |
480466, | |||
4806466, | Mar 12 1980 | The Regents of the University of California | Cell agglutination reagent comprising conjugates of antibody covalently bound to liposomes |
20070231378, | |||
20080102474, | |||
20090297534, | |||
20120070448, | |||
20120208216, | |||
20160347826, | |||
JP2008525766, | |||
JP2009142269, | |||
JP2009501713, | |||
JP2013508700, | |||
JP2015097496, | |||
JP2015145366, | |||
JP57501147, | |||
JP9506508, | |||
WO2006059904, | |||
WO9515388, |
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